FOOD AND DRUG ADMINISTRATION
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CENTER FOR BIOLOGICS EVALUATION AND RESEARCH
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VACCINES AND RELATED BIOLOGICAL PRODUCTS ADVISORY COMMITTEE
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OPEN SESSION
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THURSDAY,
NOVEMBER 17, 2005
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The
open session of the conference convened in the Versailles Room of the Holiday
Inn Select, 8120 Wisconsin Avenue, Bethesda, MD 20814, at 10:18 a.m., pursuant
to notice, Gary D. Overturf, M.D., Chair, presiding.
COMMITTEE MEMBERS PRESENT:
GARY D. OVERTURF, M.D., Chair
MONICA M. FARLEY, M.D.
RUTH A. KARRON, M.D.
PHILIP S. LaRUSSA, M.D.
DAVID MARKOVITZ, M.D.
CINDY LYN PROVINCE, R.N., M.S.N., M.A.
STEVEN SELF, Ph.D.
WALTER ROYAL, III, M.D.
BONNIE M. WORD, M.D.
FDA STAFF PRESENT:
CHRISTINE WALSH, R.N., Executive Secretary
This
transcript has not been edited nor corrected, but appears as received from the
commercial transcribing service.
Accordingly, the Food and Drug Administration makes no representation as
to its accuracy.
CONSULTANTS:
SETH HETHERINGTON, M.D.
LISA JACKSON, M.D.
PAMELA MCINNES, D.D.S.
STEVEN PIANTADOSI, M.D., Ph.D.
ROBIN ROBINSON, Ph.D.
MARK STEINHOFF, M.D.
MELINDA WHARTON, M.D., M.P.H.
I-N-D-E-X
Administrative
Matters.......................... 4
Developing New Pneumococcal Vaccines for U.S.
Licensure for Adults
FDA Presentation,
Dr. Pratt................................. 9
Opsonophagocytic Activity Assays
Dr. Steiner.............................. 35
Epidemiology of Invasive Pneumococcal Disease in
Adults
Dr. Moore................................ 51
Open
Public Hearing............................ 91
Presentations:
GlaxoSmithKline,
Inc.
Dr. Poolman........................ 92
Wyeth
Dr. Siber......................... 114
ID
Biomedical Corporation
Dr. Fries......................... 155
FDA Presentation of Questions
Dr. Gruber.............................. 188
Committee
Discussion of FDA Questions......... 184
P-R-O-C-E-E-D-I-N-G-S
10:18
a.m.
CHAIR
OVERTURF: I'd like to call the open
session back to order.
At
this point we will call the open session to order, and the first presentation
is going to be by Dr. Pratt. Before we
do that, I need to call on Christine Walsh for certain administration matters.
SECRETARY
WALSH: Good morning. I'm Christine Walsh, the Executive Secretary
for today's meeting of the Vaccines and Related Biological Products Advisory
Committee.
I
would like to welcome all of you to this meeting of the Advisory
Committee.
The
remainder of today's session will constitute of presentations that are open to
the public.
I
would first like to request that everyone please check your cell phones and
pages to make sure they are off are in silent mode.
I
would now like to read into the public record the conflict of interest
statement for today's meeting.
This
brief announcement is in addition to the conflict of interest statement read at
the beginning of the meeting on November 16th and will be part of the public
record for the Vaccines and Related Biological Products Advisory Committee
meeting on November 17, 2005. This announcement addresses conflicts of
interests for the discussion of Topic 2 on the development of new pneumococcal
vaccines for U.S. licensure for adults.
In accordance with 18 USC Section 208 B(3) waivers have been granted to
Drs. Ruth Karron and Steven Piantadosi.
A copy of the written waiver statement may be obtained by submitting a
written request to the agency's Freedom of Information Office, Room 12A30 of
the Parklawn Building.
Dr.
Seth Hetherington is serving as the industry representative acting on behalf of
all related industry and is employed by Inhibitex, Incorporated. Industry representatives are not special
government employees and do not vote.
With
regards to FDA's guest speakers, the Agency has determined that the information
provided by these speakers is essential. The following information is being
made public to allow the audience to objectively evaluate any presentation
and/or comments made by the speakers.
Dr.
Matthew R. Moore is a medical epidemiologist, National Center for Infectious
Diseases, CDC, Atlanta.
Dr.
Sandra Steiner is a microbiologist/immunologist, Division of Bacterial and
Mycotic Diseases, CDC, Atlanta.
As
guest speakers they will not participate in the Committee deliberations or will
they vote.
In
addition, there are regulated industry speakers making presentations. These speakers may have financial interests
associate with their employer and with other regulated firms. The FDA asks that
in the interest of fairness that they address any current or previous financial
involvement with any firm whose product they may wish to comment upon. These
individuals were not screened by the FDA for conflicts of interests.
This
conflict of interest statement will be available for review at the registration
table.
We
would like to remind members and consultants that if the discussions involve
any other products or firms not already on the agenda for which an FDA
participant has a personal or imputed financial interest, the participants need
to exclude themselves from such involvement and their exclusion will be noted
for the record.
FDA
encourages all other participants to advise the Committee of any financial
relationships that you may have with the sponsor, its product and if known,
it's direct competitors
That
reads the reading of the conflict of interest statement and, Dr. Overturf, I
turn the meeting back over to you.
CHAIR
OVERTURF: For this session I'd like to
call the open session again to order. And I would like to have the members of
the Committee and the consultants introduce themselves. We'll start with Dr. Wharton.
DR.
WHARTON: Melinda Wharton, National
Immunization Program, Centers for Disease Control and Prevention.
MEMBER
SELF: Steve Self, Hutchinson Cancer
Research Center at the University of Washington.
DR.
JACKSON: Lisa Jackson, Group Health
Cooperative, Seattle and University of Washington.
MEMBER
KARRON: Ruth Karron, Johns Hopkins
University.
DR.
PIANTADOSI: Steve Piantadosi, Johns Hopkins
School of Medicine.
DR.
STEINHOFF: Mark Steinhoff, Johns
Hopkins University.
MEMBER
WORD: Bonnie Word, Baylor College of
Medicine, Texas Childrens Hospital.
MEMBER
LaRUSSA: Philip LaRussa, Division of
Pediatric and Infectious Diseases, Columbia University.
DR.
ROBINSON: Robin Robinson, Office of
Public Health Emergency Preparedness, U.S. Department of Health and Human
Services.
MEMBER
PROVINCE: I'm Cindy Province, I'm the
consumer representative on VRBPAC. And
I'm with the St. Louis Center for Bioethics and Culture.
DR.
McINNES: Pamela McInnes, National
Institute of Allergy and Infectious Diseases, NIH.
MEMBER
FARLEY: Monica Farley, Emory
University, Department of Medicine, Infectious Diseases.
MEMBER
ROYAL: Walter Royal, University of
Maryland School of Medicine, Department of Neurology.
DR.
HETHERINGTON: Seth Hetherington. I'm
the industry representative and the Chief Medical Officer of Inhibitex outside
of Atlanta, Georgia.
MEMBER
MARKOVITZ: David Markovitz from the University
of Michigan.
CHAIR
OVERTURF: And I'm Dr. Gary Overturf
from the University of New Mexico School of Medicine and Chair of VRBPAC.
Our
first presentation for the open session this morning is from Douglas Pratt from
the FDA.
DR.
PRATT: Good morning. I'm Douglas Pratt from the Division of
Vaccine and Related Products Applications, Office of Vaccines, Biologics
Evaluation and Research.
I'll
begin the CBER presentation by reviewing some of the regulatory history of the
license 23 valent pneumococcal polysaccharides vaccine, PNEUMOVAX, which is
manufactured by Merck.
I
will then present a few possible scenarios for clinical efficacy studies for
adult indications with approximate samples sizes.
And
in certain situations immunologic endpoints can be used to infer efficacy for
licensure purposes. I will discuss
briefly the use of the opsonophagocytic antibody assay in this context.
And
finally, I'll discuss additional items for the Committee's consideration,
including the accelerated approval regulations.
PNEUMOVAX
23 is the only vaccine currently licensed for use in adults for prevention of
pneumococcal disease. It is made up of
23 of the most common pneumococcal serotypes that cause disease in humans. At least 90 capsular serotypes have been
identified, but 23 serotypes in this vaccine are thought to cover serotypes
that cause approximately 85 to 90 percent of invasive disease in humans.
An
earlier version of this vaccine was first licensed in 1977 as a 14-valent
vaccine that contained 50 milligrams of polysaccharide for each serotype. The vaccine was later reformulated to
include additional serotypes at reduced antigen content. The 23-valent formulation was licensed in
1983.
PNEUMOVAX
is labeled for routine use in adults over the age 50 years. This differs from
recommendations of the Advisory Committee on Immunization Practices that
recommended routine use in adults 65 years of age and older.
The
indication and use section of the PNEUMOVAX label states that the vaccine is
indicated for vaccination against pneumococcal disease caused by those
pneumococcal types included in the vaccine.
This indication does not separate out invasive disease from noninvasive
disease. And as will be shown in the
next slides, this is consistent with the primary endpoint in the support of
efficacy studies conducted in South Africa.
The
remainder of the indication in the usage section of the label is largely a
restatement of the ACIP recommendations.
Recommendations for use in immunocompetent persons two years of age and
older include persons with certain cardiac, pulmonary, liver disease, persons
with asplenia and persons living in special environments.
Recommendations
are also made for persons older than two years with immunocompromising medical conditions.
Studies
conducted in South Africa by Schmidt and colleagues provided the principal
basis of efficacy for the polysaccharide vaccines at the time of
licensure. Results of two South African
studies, one using a 6-valent vaccine and another subsequent study using a
12-valent vaccine were provided in the license application.
Efficacy
results for the 12-valent vaccine are show in this slide. Note that the mean age for subjects in this
study was 22 years. Duration of follow-up for case ascertainment was
approximately one year.
The
primary endpoint was pneumococcal disease due to vaccine serotypes.
Confirmation of vaccine serotype was by blood, sputum or nasopharyngeal culture
or by mouse inoculation. And the study
report stated that sputum was the sample used in the mouse inoculation
test. In fact, in the study none of
these cases from any of the study groups was confirmed by a blood culture.
The
efficacy estimate, 91.7 percent, was determined by comparing against the
combined placebo meningococcal A&C vaccine controls. Noteworthy is the attack rate in the
control groups which exceeded 22 per 1,000 or 2200 per 100,000.
Two
serotypes were subsequently added to the 12-valent formulation prior to
licensure of the 14-valent.
Well,
after licensure of the 14-valent vaccine pneumococci of other capsular
serotypes were recognized as important causes of pneumococcal disease. The manufacturer was asked to reformulate to
include additional important serotypes.
Due
to concerns about the amount of bacterial polysaccharide in a 23-valent
product, formulations of lower polysaccharide antigen content were
studied. In the study submitted to the
license application to support the formulation change, healthy subjects 21 to
64 years of age received a 22-valent product containing either 50 or 25
micrograms per serotype. The immune
response were determined by a 2-fold Rise in the antibody titer is measured by
radioimmunoassay. Responses of the two
groups were judged as essentially the same and the safety profile was also
judged as acceptable.
Prior
to licensure Type 33F was added to the license formulation.
Well
as noted previously, the supportive efficacy studies for the polysaccharide
vaccine were conducted in young South African gold miners. Among the elderly and other high risk groups
studies have yield mixed results.
Provided in the briefing materials for the Committee as copies of
reviews with meta-analyses discussing some of these results.
The
ACIP recommendations for routine use in persons older than age 65 is based on
case control studies evaluating invasive disease citing effective estimates
that range from 56 to 81 percent.
Effectiveness
for non-bacteremic disease in the elderly has not been convincingly
demonstrated. Again, the ACIP statements
cites a lack of specific and sensitive diagnostic tests for non-bacteremic
pneumococcal pneumonia as a possible reason for the inability to detect a
vaccine effect.
While
it's not my intention to discuss exhaustively the various studies and results
regarding the effectiveness of the polysaccharide vaccine, but two relatively
recent studies addressing efficacy for groups included in the ACIP
recommendations and in the labeled usage section of the label deserve mention
and are cited on this slide.
In
a large retrospective cohort study of more than 47,000 persons over age 65
conducted by Dr. Jackson and colleagues, effectiveness of the vaccine and
preventative invasive disease was estimated at 44 percent. However, no effect on all cause pneumonia
was demonstrated.
In
a randomized controlled trial conducted in Uganda among adults infected with
HIV, the vaccine was ineffective against invasive disease and all pneumococcal
outcomes. And, in fact, was associated with a significant increase for all cause
pneumonia.
Prospective
randomized control trials provide the best evidence of clinical
effectiveness. The choice of efficacy
endpoints for any vaccine and the clinical efficacy trial should be guided by
what is most clinically meaningful.
Clinical endpoints in vaccine trials should provide evidence of benefit
to the individual. Thus, indirect
effects such as hurt immunity have not been used as a primary basis of
efficacy.
Also
cost effectiveness outcomes are not endpoints suited for regulatory decisions.
Feasibility
of the studies in terms of cost is not a judgment for FDA, although FDA
reviewers recognize the practical issues associated with the choice of
endpoints. Vaccine manufacturers and
sponsors of the vaccine trials will ultimately decide the kinds of studies that
are feasible from their perspective.
Well,
in thinking about possible clinical trial designs to establish efficacy of a
new pneumococcal vaccine in adults, age of trial for participants requires
careful consideration. Adults over the
age of 65 years are considered high risk of pneumococcal disease and so
represent one of the most relevant populations in which to determine vaccine
effectiveness. However, because the
polysaccharide vaccine is recommended for routine use in all persons over age
65, it might be considered unethical to withhold or delay vaccination with the
licensed vaccine in order to conduct a randomized placebo controlled trial in
this population.
The
age group of persons 50 to 64 years old is at moderately high risk for
pneumococcal disease. And this group also includes individuals with other risk
factors that put them at high risk. A
placebo controlled trial in this age group may be feasible and would not be
associated with the same concerns about withholding a recommended vaccine. However, an efficacy study in this
population may not accurately predict effectiveness in the higher risk groups.
A
few scenarios of possible clinical endpoint studies are presented in the slides
that follow. Each of these scenarios considers persons 50 to 64 years of age in
placebo controlled studies. Endpoints
considered include invasive pneumococcal disease, all cause community acquired
pneumonia and presumptive pneumococcal pneumonia.
A
number of assumptions are necessary to estimate the sample sizes and different
statistical programs may yield different sample size estimates. To construct
these scenarios it was assumed that studies were placebo controlled, randomized
one-to-one and studies would provide for a mean follow-up of 22 years per case ascertainment.
Also
within each scenario sample sizes are provided for a vaccine with serotype
coverage of about 60 percent, which might approximate a conjugate vaccine
coverage another set of sample sizes for a vaccine with more broad coverage,
such as is provided by the 23-valent vaccine.
Ninety
percent power was used to manage the risk of a failed study due to inadequate
sample size.
Well
critical to the sample size calculations is the expected background rate of
pneumococcal disease. For this scenario a lower rate of 25 per 100,000 was
chosen. This approximates a rate of 20 per 100,000 cited by Whitney et.al. in
2003 for a wider age range of 40 to 64 for adults in the U.S. Of course, the
epidemiology in the U.S. continues to change, as well be discussed later by
Matt Moore of CDC.
A
higher rate is also presented 50 per 100,000 because it may be possible to
identify populations with other risk factors such as smoking history, asthma or
membership in a high risk ethnic group or which identify populations outside
the U.S. with higher rates of pneumococcal disease.
This
table provides the estimates sample size per group for the various assumptions.
These values are not intended to be precise, but only to provide an idea of the
scale of the studies that would be required.
To walk through an example at the top of the table for an assuming of
the lower background rate of 25 per 100,000 due to all pneumococci, and
assuming 60 percent vaccine coverage with a true efficacy of 70 percent, the
study would require 82,000 subjects per group.
And
at the other end of the spectrum using a higher background rate of 50 cases per
100,000 with a broader vaccine coverage of 85 percent and true vaccine efficacy
of 90 percent each group would require 16,000 subjects.
It
can also been seen that doubling the background rate reduces the sample size by
half for the scenarios that are otherwise the same.
All
of these efficacy estimates have relative robust 95 percent lower limits on
efficacy which are well above zero excepting a lower lower bound prolonging
follow-up for case ascertainment and broadening the serotype coverage would all
lower the samples sizes for this endpoint.
Typical
vaccine efficacy studies have used specific case definitions that rely on
identification of the disease causing pathogen, usually by culture
methods. Such definitions provide high
efficacy estimates for effective vaccines.
So called effectiveness trials evaluate less specific endpoints for
which the pathogen is not identified. A
relevant example for our discussion would be the endpoint of all cause
pneumococcal pneumonia.
Effectiveness
studies have supported vaccine indications in the past and a relevant example
was the effectiveness trials supporting an indication for the approval of Flu
Mist for adults 18 to 49 years of age.
The indication for use in adults was based on clinical definitions
consistent with the diagnoses of influenza but not confirmed as influenza by
virus culture. Note the efficacy estimates of 11 to 24 percent for prevention
of these influenza syndromes.
These
data were judged adequate to support the use of FluMist in adults 18 to 49
years of age, however for this vaccine efficacy had also been demonstrated for
culture confirmed disease in young children.
So
in this second scenario an effectiveness endpoint of all cause community
acquire pneumonia is considered a background of community acquire pneumonia of
300 to 600 per 100,000 is used. Data on
community acquire pneumonia in this age group is actually difficult to
obtain. These numbers are based on a
study by Marst et.al., a study in Ohio for the age range of 40 to 64 years of
age, and then rounded upwards slightly to 300 per 100,000 for the 50 to 64 age
range.
A
similar background rate can be estimated by back calculating from the rate of
invasive disease, assuming four to five cases of pneumonia for each case of
invasive disease, and that about 30 percent of all pneumonia resulting in
hospitalization is due to pneumococcus. Using other assumptions as before,
these are the sample sizes that would be required.
The
derived efficacy estimates for all cause pneumonia are low as expected here
ranging from 30 to 23 percent.
Sample
sizes are quite large for some of these assumptions. Nevertheless, such studies might be feasible in populations with
higher background rates and with a vaccine with broad serotype coverage. Such studies could be conducted simply by
making use of automated databases and should not be resource intensive.
Well, identifying pathogens causing
non-bacteremic pneumonia with a high degree of certainty can be difficult. Isolation of pneumococci from the upper
respiratory tract is not a guarantee that the bacteria is causing lower
respiratory tract disease as pneumococci can be part of the normal upper
respiratory flora. Nevertheless,
clinical radiologic and microbiologic information guide treatment of suspected
pneumococcal pneumonia in the clinic.
And as note earlier, the bulk of the data supporting efficacy of the
original South African gold miner studies in pneumococcal disease and pneumonia
confirmed by culture of the sputum.
Using
additional diagnostic modalities, it seems likely that the specificity of the
diagnoses can be increased. A
commercially available urine antigen test for pneumococcal C polysaccharide is
reported to be highly specific with respect to blood, sputum and nasopharyngeal
culture when used quantitatively.
Other
urine tests specific for individual pneumococcal serotypes are under investigation.
Nonspecific
markers of information such as C-reactive protein and procalcification have
also been proposed as measures to improve the specificity of a diagnoses of
bacterial pneumonia.
With
a precise amount that the specificity of the diagnoses can be increased by
these auxiliary methods is not clear, and we choose not to account for the
specificity in the sample size estimates that follow.
Let
me back up to get to the background rate used in this scenario. The background rate of 100 to 200 cases per
100,000 is used. This is based on estimating one-third of the hospitalizations
due to community acquire pneumonia in the previous scenario would be to
pneumococcus. And then again this rate
can be arrived at by back calculating using the similar assumptions from the
rate of invasive disease.
So
these are the sample size estimate for an efficacy trial for an outcome of
presumptive pneumococcal pneumonia.
Lower efficacy might be expected for pneumonia compared bacteremia, so
assumed efficacy was lowered in these estimates to range from 60 to 80 percent
as opposed to 70 to 90 percent of this table.
A true efficacy of 90 percent would require smaller sample sizes.
Low
sensitive and low specificity for the diagnoses would tend to increase the
sample size. Higher background rates of pneumococcal pneumonia, more broad
serotype coverage and longer follow-up for cases and a less stringent lower
bound on the efficacy estimate would reduce the sample sizes.
Due
to the diagnostic workup and logistics of such a study it could be relatively
more recourse intensive per subject than the previous scenarios.
Some
concepts for trails in older adults are outlined in the following two slides,
as discussed previously conducting placebo controlled studies in the
elderly might be difficult, in part,
because of the ethical concerns about withholding a recommended vaccine. And it's not clear that any of these studies
could be done. However, in a well
monitored study a decision to delay vaccine with the polysaccharide might be
viewed as acceptable by IRBs and subject given that the current recommendation
is to give polysaccharide vaccine only once.
There's some uncertainty about the efficacy in this age group and if concerns
about hyporesponsiveness following the polysaccharide vaccine are valid. Background rates of disease are higher in
this population, so sample sizes would be smaller, studies more feasible and
this is certainly a relevant population to study a vaccine.
So
the first scenario would be a placebo controlled study of the new vaccine
against a placebo.
The
second scenario, the second concept for a new vaccine would be to add the new
vaccine onto a background of 23-valent vaccine in an attempt to assess added or
the existing therapy. Such a study would not have the ethical concern about
withholding or delaying vaccine with the 23-valent polysaccharide.
For
an invasive disease endpoint sample sizes could be prohibitive since
polysaccharide vaccine is effective in this population. However, since efficacy
of the polysaccharide vaccine for non-bacteremic disease is apparently quite
low and possibly similar to placebo, comparative studies to evaluate
non-bacteremic disease might be feasible. And this would, certainly, be a
highly relevant outcome.
And
the third design concept to new vaccine would be compared head-to-head against
the 23-valent polysaccharide vaccine.
For a low efficacy estimate such studies would be quite large.
And
then in a fourth design for consideration, this would be a three arm study that
combines concepts one and three. It
would be powered to provide stand alone efficacy relative to placebo and would
have the 23-valent polysaccharide as a control to check against unexpected
outcomes such as a lower efficacy than might be expected for the license
vaccine alone. But we do not attempt
sample size calculations for these additional four scenarios, and they're
presented here for your consideration.
In
certain situations efficacy of a new vaccine can be inferred from an immune
response that is similar to that induced by a licensed vaccine for which
efficacy has been demonstrated. A
recent example of this approach was the licensure of Menactra, a quadrivalent
meningococcal conjugate vaccine which was approved based on immunologic
non-inferiority compared to the licensed polysaccharide vaccine Menomune, both
of which are manufactured by Sinofi Pasteur.
Such
an approach is also consistent with advice provided by the 2001 VRBPAC
regarding approval pathways for new pneumococcal conjugate vaccines in
infants. For infants, the comparative
assessment of antibody concentration using a standardized ELISA was judged
acceptable. However, antibody levels
that may be useful in children for non-inferiority comparisons for inferring
efficacy would likely not be valid for adults, many of whom have preexisting
antibody to some or most serotypes. And
the level serum antibodies that correlate with protection in adults and elderly
have not be determined.
Evaluation
of an effective immune response in adults is thought to be more dependent on
serum opsonophagocytic antibody titers.
Opsonophagocytic
antibody is a measure of functional antibody that is thought to be central to
protection against pneumococcus for vaccines directed at capsular antigens. Details of the assay will be discussed later
by Dr. Sandy Steiner, but in brief antibody lining to the bacterial surface
with complement is taken into phagocytic cells and a serum titer of
opsonophagocytic antibody can be determined in this assay. The in vitro assay is thought to provide
evidence of in vivo protection. However, some unknowns remain. Protection from
disease will depend not only on function of the antibody, but also function of
the phagocytic cells. And it's not clear that the phagocytic cells of the
elderly and other high risk populations will function similarly to the cultured
phagocytic cells used in the assay.
Also,
the quantitative relationship of the OPA that correlates with efficacy as
determined in clinical trials has not been established. It's also the quantitative relationship may
differ by disease endpoint; that is the amount of antibody needed to protect
against an invasive disease may differ from the amount of antibody needed to protect
against pneumonia.
With
a regulatory pathway using demonstration of non-inferior immune response to
that of a licensed vaccine is problematic when the new vaccine has fewer
serotypes. Evaluation for common
serotypes could actually be straightforward, but the comparison to the licensed
vaccine, the new vaccine would fail on comparisons to those serotypes that are
only in the 23-valent vaccine. One is
left with the problem of how to account for the serotypes that are not included
in the new conjugate vaccine but present in the polysaccharide vaccine if one
follows the pathway of comparison to the licensed product.
Well,
to compensate for fewer serotypes it may be argued that the conjugate vaccine
offers theoretical advantages of the superior immune response over that of the
licensed product for serotypes in common.
Such higher antibody levels that are opsonophagocytic antibody activity
or lack of hyporesponsiveness. In this
regard criteria for demonstrating a superior immune response have not been
developed for regulatory purposes. It's not clear how much additional
opsonophagocytic antibody would be needed to be meaningful. Evidence is lacking that higher antibody
levels of OPA result in greater protection.
A
regulatory decision to attribute vaccine benefit based on an immune response
that is superior to that induced by the licensed vaccine would be a novel
approach to licensure, and this approach would need scientific consensus and
VRBPAC advice.
Conjugate
vaccines would still need to be used in conjunction with the 23-valent vaccine
to assure immunization for all 23 types in the 23-valent vaccine. Use of the conjugate vaccine in conjunction
with the 23-valent vaccine would raise some additional regulatory concerns,
such as how the vaccines would be labeled. There are specific regulations
addressing labeling of products to be used on combination.
Also,
if a conjugate vaccine is to be used before a polysaccharide vaccine, that
could have labeling implications for the licensed product, PNEUMOVAX, and it's
also uncertain what the regulatory status of the new product would be if for
some reason the 23-valent vaccine were to become unavailable and whether
additional studies would be needed at that point in time to support a stand
alone licensure.
Well,
for vaccines targeting noncapsular antigen an immunologic efficacy is not
possible since preventative efficacy of these new vaccines has not yet been
demonstrated. Also, it's not clear if
they will be able to induce functional antibody. Thus, it appears that a clinical endpoint efficacy study will be
needed for vaccines targeting noncapsular antigens. With broad serotype coverage anticipated from such vaccines
clinical endpoint efficacy studies would be more feasible.
Indirect
effects of vaccination after introduction of Prevnar are thought to be due to
prevention of colonization and carriage in the nasopharynx of children
resulting in reduction of transmission to older adults. Clinical studies
designed to evaluate colonization would provide clinical evidence of a vaccine
effect. However, since colonization is an asymptomatic condition it's
prevention offers no direct clinical benefit to the vaccine participant.
Prevention
of colonization or carriage has not previously been used as a primary clinical
endpoint to support licensure decisions.
Use of nasopharyngeal colonization or carriage as the primary efficacy
basis of approval would need acceptance as a surrogate of efficacy. Studies to evaluate nasopharyngeal
colonization, however, would likely be feasible.
Finally,
I'd like to talk a little bit about the accelerated approval regulations. Accelerated approval regulations provide a
regulatory option for certain products intended to treat or prevent severe and
life threatening conditions. Under the
accelerated approval regulations a product can be approved based on a surrogate
of efficacy. The level of evidence
required of the surrogate is that is reasonably likely to predict clinical benefit. The new treatment must offer meaningful benefit over existing
treatments.
Another
necessary condition under accelerated approval is that a confirmatory clinical
study, clinical endpoint study validating the surrogate must be conducted
post-licensure. Confirmatory studies
should be well underway at the time of the accelerated approval.
The
accelerated approval regulations have been used only once in vaccine
development, and that was for the recent approval of Fluarix, trivalent
inactivated influenza vaccine made by GlaxoSmithKline. Hemagglutination inhibition antibodies
served as the surrogate in that case.
It
seems likely that pneumococcal conjugate vaccines for the elderly could meet
the conditions of accelerate approval using opsonophagocytic antibody as a
surrogate.
So
in summary new pneumococcal vaccines for use in adults and the elderly are
being developed by multiple manufacturers.
Evidence of effective to support licensure might be based on clinical
endpoint efficacy studies or immunologic criteria such as opsonophagocytic
antibody.
Advice
of VRBPAC is being sought regarding the most appropriate endpoints, trial
designs, study populations to support licensure of a new pneumococcal vaccine
for adult indications.
And
I'd like to acknowledge my colleagues.
CHAIR
OVERTURF: There will be time for
questions after three presentations, so we will hold those questions at this
point and proceed to the next presentation, which is Sandra Steiner on
opsonophagocytic activity.
DR.
STEINER: Good morning. Thank you very
much for the invitation.
I
hope to talk to you about the functional antibody activity as measured by
opsonophagocytosis.
At
any given point in time the host, the human host, can a variety of antibodies
present in circulation that are specific to pneumococcus. They can be present there by a number of
factors; either through disease, vaccination, passive immunization,
colonization or possibly through cross reactivity.
In
the laboratory we measure those antibodies by a variety of methods. The ones that you're probably more familiar
with is the ELISA method that gives you a microgram for a concentration is a
quantitative measurement. However, we
wonder how those antibodies actually work and do they actually confer some
protection.
We
have terms these concept functional antibody activity and there are functional
determinations that are performed in the laboratory to measure these. One of them is animal protection studies
where you do passive protection studies, and they're very difficult for those
large trials that you have seen the numbers earlier on today.
The
other one will be opsonophagocytosis, which I will explain in a bit of detail
later on.
There
are also indicators of memory that are used and these indicators are probably
more important for the conjugate vaccines where you hope to have some prime --
and they are measured by antibody avidity.
The antibody avidity is a modified ELISA assay. And you can also measure them by checking
B-cells and finding out how well they assimilate when they encounter the
antigen once more. And this is done by ELISA assays.
Concentrating
on opsonophagocytosis and we can try to get the concept if we actually look at
these two slides. Without the presence
of antibody, you can see that the diplococci, the pneumococci are outside of
the phagocytic cell. But in the presence
of antibody these diplococci, the pneumococci actually get engulfed and they
are present inside the phagocytic cell.
When they're inside the cell, they're actually killed because they
cannot survive inside that phagocytic cell.
So
we need to find out how do we measure these and which are the players that
actually carry out these functions inside the host. We have here the phagocytic cell that has a number of receptors
on the surface for immunoglobulins and for complement. And the opsonins and the
target bacteria. The bacteria will have
a capsule on the surface that is specific of the serotypes, depending on what
code they have on. The antibodies bind
specifically to the surface of that capsule.
And then once they bind, the complement will be deposited onto the
surface of that bacteria. These
bacteria is now opsonized and once it's opsonized it's very amenable to that
phagocytic cell. They will be engulfed.
And once it is engulfed, it will be inside the phagocytes so many will be
killed.
So
about 12 years ago we started looking into a standardized way of doing this
type of looks in opsonophagocytic assays.
And we published a methodology for a single serotype measurement in
which four components are present: The
serum where you try to find out the function of those antibodies; the target
bacteria; complement is one of opsonins, and; the culturable phagocytes which
in our case we have been using HL60 cells differentiated into a
polymorphonucleic cells.
As
I mentioned before, once the pneumococci are internalized they are killed and
what we actually measure is an opsonophagocytic titer.
In
the laboratory when you're trying to determine these titers what you have is a
series of unknowns serum that are run in duplicate. They are diluted, serially diluted
and you have a quality controlled serum and immunoglobulins that are used as a
reference. It is a gamma globulin
preparation.
And
what you do is you look at the killing that each of the samples will give and
you compare it to the complement controls. Then you carry out the determination
of the 50 percent or the dilutions that can give you at least 50 percent
killing for the target period. And what
you get are various titers being determined.
It depends on what amount of antibodies are actually functional inside
that serum sample how that titer varies.
Once
you determine all those points for the various serum, what you have is a curve
that you can actually draw. And you can
do this by more advanced analytical analysis, like four parameter logistic
curve regression analysis. This was
data present by Tom Taylor in the lost pneumococcal meeting that we had in June
of 2005. And there you can actually see
that you can actually fit a curve that goes with the whole inflection. You can determine the midpoint of the curve
and a continuous titer could actually be determined as well as you could also
report a discontinuous titer.
So
this particular assay has been developed as a single serotype assay. But it's time consuming and is very reagent
demanding. So efforts from Dr. Moon H.
Nahm at the University of Alabama and in the Netherlands a Dr. Peter Hermans
have allowed us to have a variety of other tests available that have two, four
and up to seven different serotypes that can be measured simultaneously.
These
are results presented at the pneumococcal meeting in June of 2005 by Mr. Burton
where we have a correlation of the single serotype of opsonophagocytic assay
with assays that were run simultaneous for four different serotypes in a
multiplex format using viability as an endpoint. As you can see, there is a very good level of correlation for all
the four serotypes that were tested.
And there were probably two outliers or outside of the confidence
interval, but overall the correlation is good, especially if you don't consider
that particular outlier seen there.
They
have also spent a great effort working on the automation of these assays. And we don't want to do these counts,
because they're very difficult to do manually.
So they've worked on getting equipment that can actually do the counts
in a fast throughput manner and be able to collect the data and graph it to be
able to calculate the titers in a more speedious way.
We
have also been working on eliminating the counts altogether. And we just
recently published on a florescent methodology that we'll be able to eliminate
the counts. And it's also done in a single and a multivalent format. These were using the strains that Dr. Debbie
Bogaert had published in the Netherlands in her study from 2004.
There
are a number of other assays that are also available for
opsonophagocytosis. And we term them
for convenience the update of opsonophagocytic assays.
The
uptake OPAs are primarily through flow cytometric methods and they measure the
uptake of kill bacteria or polysaccharide coated particles. They can be available in a single serotype
or in a multivalent format also with up to four different serotypes measured at
the same time.
The
flow cytometric assays do target a population of the effected cells, so you're
actually looking at the phagocyte. And
then you look at the shift in the fluorescence of that population of cells to
the right once they have been uptake of the fluorescent particals. So that generates a curve of data similar to
the ones that we had for the killing assay.
And you can also calculate the 50 percent point and determine the titer.
Again,
as I mentioned, I could be done in the monovalent format, I mean has it various
levels of correlation to the single serotype assay, viability assay or in a
multivalent format.
So
you're probably wondering what is the current validation status of all these
assays. And for the single serotype
killing assay, I'm glad to say that we have developed standardized, evaluated
and validated at the GLP level thanks to the efforts of the entire scientific
community.
For
the other assays it's a different story. They have only been developed and
standardized. So there's a lot of work
to be done there, especially to be able to multiplex.
Some
of the data that I will be giving you later on is related to the efforts that
lead to the evaluation and validation of the single serotype of
opsonophagocytic assay. These are
results from a laboratory evaluation that we did once the technology was
transferred to the various laboratories across the world. And they participated
in a multi-laboratory evaluation with a panel of quality control sera that was
evaluated for at least seven different serotypes. We counted exceptions that are highlighted here in yellow. Most of the sera were overall with a 75
percent branding only one dilution away from the median titer. And 88 percent of them were two dilutions
away from the median titer.
When
we look at how well were those titers being hit depending on the sera type, the
particular sera type or depending on the titer, I'm just giving you here the
results for serotype 14. We noticed
that it was easier to get an agreement between laboratories if the titers were
low. Right here is a titer of only
four. But if the titers are higher,
then there is more of a variability along each of the serum samples with the
defined titer that is being reported.
So it's harder to hit higher titer than a lower titer.
The
validation efforts have been done primarily by industries, since they have been
able to apply this technology in their hands. And this is studies that was just
recently published by Brenda Hu from Wise Laboratories. And they have been able to report the
specificity of the assay to be greater than 80 percent. And notice that only a
heterologous Ps could only give less than 20 percent reduction of the
signal.
The
intermediate precision was determined to be overall 81 percent for all the
titers to be 2 dilutations away from the median.
And
the linearity for 9 serotypes evaluated was fairly good, between .98 with very
good slopes, also around 1.
The
accuracy for nine serotypes was 100 percent for seven of them, but for two of
them it was slightly lower.
And
overall, they determined that the assay was fairly robust.
And
maybe what you have been waiting for is how is this correlating with
protection. I will give you selected information that is more related to how we
have derived these to be a potential correlate for protection.
The
ELISA correlation in healthy populations, the passive protection in animals and
the minimum level needs for vaccine efficacy in infants as follows, and I will
give you a little bit on the elderly what we know.
For
the ELISA, these are results of the adults following 23-valent polysaccharide
vaccine, recipients of that vaccine. And we see a correlation between ELISA and
opsonophagocytic titer that is fairly high. This is all serotypes
combined. You will be able to see
results like these for many, many studies that are present in the
literature. And the correlation is very
good in infants. And as you start
working with normal healthy adults, but as you start working with populations
that are more at risk and the very
elderly the correlation with ELISA is not as good.
The protective level in mice that was
determined in a study presented by Johnson in 1999 demonstrated that you could
protect against non-bacteremia.
Seventy-five of the mice could be protected against bacteremia with a
titer, a opsonophagocytic titer of eight.
And
this is a study from infants and is based on the Northern California Kaiser
Permanente trials for the vaccine. And in this particular graph you can see a
reverse cumulative distribution of children that have had an antibody
concentration involve a particular level that is listed in the X axis.
And
what we can see here is that 97.9 percent of the vaccinated population had at
least .2 micrograms per mil in concentration in their serum while only 12.9
percent of the control population had that particular titer.
This
study was also used to help compare the values with the opsonophagocytic titers
and help us define what will be the minimum opsonophagocytic titer. And in here you can see the correlation
between the ELISA concentration -- I apologize for that. And the opsonophagocytic titer. And what you can see in these quadrants is
at .2 micrograms per mil concentration actually corresponds to a titer of 8.
And that discriminates clearly between the recipients of the conjugate
polysaccharide vaccine and those that are the controls. This study was published by Jodar in 2003 in
Vaccine. However, this is a minimum value with a correlate of for
opsonophagocytosis only in infants.
What
do we know about dysfunctional antibodies in the elderly? The studies are being performed right now
and a lot of these studies actually have not been published yet. But for what I can tell you is that the
protected levels are unknown, as you heard in the first talk, too. That we
don't know the ELISA or the opsonophagocytic titer that will actually
correspond to protection in elderly or in other populations at high risk.
We
did study in 1999 before ELISA had absorption of antibodies where we found that
there was a reduction in the function of the antibodies that were eliciting the
elderly after receiving the pneumococcal polysaccharide vaccine 23-valent. And the reduction was more notorious or more
prominent in the very, very elderly; people that were 80 to 89 years of age and
if they were greater than 90 years of age.
We attributed these to a lower avidity in the antibodies. And we saw a
very poor correlation with ELISA with the exception of serotypes 14 where we
had a .8 correlation. And these
antibodies did not protect in mice.
In
the year Usinger and Lucas did a very elegant study with avidity and function.
And they also looked at adult serum with polysaccharide vaccine and they
confirmed the relationship between avidity and function and that you're
required to have high avidity in the antibodies in circulation to be able to
have function, opsonophagocytic function in those antibodies. Those antibodies will be the ones that will
protect in mice.
And
just recently we with the collaborators in Toledo, Ohio, Dr. Westerly Slabb,
we've been able to show that in elderly a lot of those antibodies are cross
reactive. And when you absorb them with
additional -- the absorption -- like with 22F polysaccharide, you can reduce
the signal that is being measuring the ELISA.
And that they still produce opsonophagocytic activity in the elderly, in
this case where people higher than 77 years of age.
We
need very large scale studies that can address and look at all these issues.
And I know some of these studies are underway, and probably very soon to be
published. So, hopefully, we will have
more information available.
The
clinical studies that have used these opsonophagocytic assays are mostly
outside of the U.S. have been done by the Finns. As these are results from presentations that Nina Ekstrom presented at the pneumococcal
meeting in June 2005. And without going
into detail in all of them, you will be able to see that they have evaluated a
lot of the conjugate vaccines that are being worked with for trials. And they
work in Finnish children, in African, in populations in Israel, and also in
Filipino populations. And they've used
primarily the killing of opsonophagocytic assays single serotype, but they also
are starting to use the flow cytometric opsonophagocytic assay in some of their
trials.
So
here are advantages of what we are doing here with opsonophagocytosis is
because we will have a laboratory correlate of protection. And it could
potentially reduce the numbers of efficacy studies that need to be done. And also we have a method available that has
been worked out all the way to the GLPs or the good laboratory practice level
that is the killing single serotype OPA.
We
have information about the assay and strains and references available at the
website that is maintained by Dr. Moon H. Nahm at the University Alabama. He has standardized, validated. He used culturalable phagocytes to eliminate
the variability between donors.
His
high throughput can be done at high performance conditions and it can be used
for data analysis that is more sophisticated.
The
disadvantages of using an opsonophagocytic assay, of course, is no matter what
we face still in vitro correlate. And
it requires laboratory facilities, the training of technical staff. And we need
a lot of information regarding multiplex assays before they can be used for
these type of assays for studies.
Thank
you very much.
I
would like to give thanks for inviting me here today and to all of my
colleagues at CDC for helping me with this.
Thank
you.
CHAIR
OVERTURF: Thank you.
We'll
proceed with the last presentation of this morning, which is Matthew Moore.
DR.
MOORE: Good morning. I'd like to thank the Advisory Committee for
the opportunity to talk with you this morning about the epidemiology of
invasive pneumococcal disease in adults.
I
think before I get too far into that, I need to spend a little time talking
about the epidemiology in children because I think it's very instructive in
helping us to think about or to construct a framework for thinking about the
effects of a new vaccine in adults. So
first I'm going to review the direct effects of the seven-valent conjugate
vaccine in children both in terms of the direct effects and then the
indirect. And I'm also going to talk a
little bit about replacement disease.
Then I'll move on and talk about the indirect effects of PCV7 among
adults by age group, by syndrome and by underlying disease status. Toward the end I'll get in a little bit to
what we might expect in terms of serotype coverage in adults for different
conjugate vaccine formulations as well as the 23-valent polysaccharide
formulation. And then I'll just end
very briefly on opportunities for evaluations of new vaccines in adults.
So
let's talk about children first. Many
of you in the room are familiar with this surveillance program called Active
Bacterial Core Surveillance or ABCs. This is a laboratory-based,
population-based surveillance system that operates in several areas around the
country. For the purposes of this discussion
I'm going to focus on the areas highlighted in yellow here which were under
continuous surveillance from 1998 through 2004. And although some areas are highlighted in their entirety, I
should point out that for example in the state of California it's really only
one county that was under continuous surveillance. The state of Connecticut, on
the other hand, was under continuous surveillance for the entire state for this
whole period.
ABC's
methods are relatively straightforward although pretty labor intensive. Our case definition includes streptococcus
pneumonia isolated from a normally sterile site, such as blood as cerebral
spinal fluid.
For
each case a chart review is performed, and this is a very labor intensive
process that's conducted by our state health department and our academic
partners.
The
epidemiologic data are aggregated at CDC, but then the individuals isolates are
also sent to reference laboratories for serotyping, susceptibility testing and
genetic testing using a method called multi locus sequence typing which I'll talk
about in a few minutes.
For
the purposes of this discussion I'm going to spend a lot of time talking about
rates of disease expressed as cases per 100,000 population broken down into
these age groups highlighted in yellow.
Again, this is going to be using the sites that were under continuous
surveillance from 1998 through 2003, which is approximately 17 million persons
in the U.S. All of these changes are
going to be expressed as percentage increases or decreases with 95 percent
confidence intervals so you can get a sense of what is statistically
significant.
At
the end I'll talk a little bit about the vaccine type invasive disease cases
that were directly and indirectly prevented based on these data.
So
this is the first slide showing along the X axis the calendar year of
observation and along the Y axis the incidents of invasive pneumococcal disease
in children under the age of 18.
The yellow line at the top highlights children
under the age of 5. Obviously, these were targeted for vaccination. And the
green line way at the bottom indicates children aged 5 through 17.
You
can see that in 2001 the vaccine was introduced and following that there was a
77 percent decline in invasive pneumococcal disease in children under the age
of 5 from 1988 through 2004.
In
older children, age 5 to 17, there was a 42 percent decline, and this was also
statistically significant. So the next
question might be well how much of this is actually attributable to the
7-valent conjugate vaccine? And one way
to get at that question is to only look at rates among those serotypes
contained in the vaccine. And that's
what this slide shows. Notice that the
scale on the left has gone from 120 cases per 100,000 at the top to about 90
cases per 100,000. So the majority of
those cases we were seeing in children under the age of 5 were, in fact,
vaccine serotypes. But now we see a 97
percent decline in the rate of invasive disease among children under the age of
5 with very narrow confidence intervals.
Even
among older children, however, we saw a decline of 75 percent. And, again, this
was statistically significant.
Well
another question might be what about those serotypes that are not contained in
the vaccine themselves but are, in fact, related to the serotypes contained in
the vaccine. And these would include
things like 6A, 9A, 9N, etcetera.
This
slide shows the rates of invasive disease caused by those vaccine related
serotypes, excluding serotype 19A. And
that will become evident in a minute why I've excluded that.
In
children under the age of 5 we saw an 92 percent reduction in the incidence of
invasive disease caused by these vaccine related serotypes. In older children we saw no statistically
significant change.
What
about non-vaccine serotypes, so those that are not in the vaccine and are not
related to the vaccine? In children
under the age of 5 we actually saw a 64 percent increase in the rates of
invasive disease caused by non-vaccine serotypes. So this is replacement disease, and this is what we concerned
might happen.
In
children aged 5 to 17 we saw no statistically significant change and the rates
were pretty much flat.
Well,
remember a minute ago I told you that I was excluding serotypes 19A, and this
is why. Serotype 19A has turned out to
be the prominent replacement serotype among children under the age of 5. Between 1998 and 2004 we saw a 194 percent
increase in the incidents of invasive disease caused by serotype 19A. I draw
your attention, however, to the Y axis which peaks out at least in 2004 at
about 8 cases per 100,000. So although
in relative terms this is a substantial increase in the rate of serotype 19A
disease compared to the huge decrease that we saw in overall disease and the
even larger decrease that we saw in vaccine serotype disease, this is still a
relative moderate increase.
Well,
how did 19A become so common? I think this may have implications for future
vaccine development. One hypothesis is
that perhaps a new serotype 19A clone was introduced into the population,
either from an area in the U.S. in which we're not doing surveillance or
perhaps from another country.
Another hypothesis is that one or more of the
7-valent serotypes actually switched their capsules to become serotype 19A. So
how can we try to address these two hypothesis?
This
is where we get int our genetic testing using multilocus typing. This is a molecular typing method which
determines the degree of genetic relatedness independent of the capsules
serotype. It's based on the DNA sequences of seven "host keeping
genes" which are relatively preserved in the pneumococcus over time. Each
of these sequence types is assigned to a clonal complex or a family. Sometimes we call them clonal clusters.
So
this pie chart on the left shows in 1999 among children under the age of 5 with
serotype 19A invasive disease there were three different clonal clusters. The numbers clonal cluster 199, 81, 1665 are
pretty arbitrary. The point of this pie
chart is to show you that in 1999 there were really only three clonal clusters
that accounted for all of the serotype 19A disease in young children.
If
we were to think that perhaps a single clone came in and caused the increase in
serotype 19A disease, what you would expect is that this pie chart would change
by having just one additional section or color added to it. In fact, in 2003/2004 we've seen multiple
new clonal clusters introduced into the serotype 19A population. Why did this happen?
Well,
this same pie chart I've just moved over to the left side of this screen if the
serotypes contained in the vaccine were switching their capsules to become
serotype 19A, then you might think back in 1999 those serotypes might have been
associated with other clonal clusters. And, in fact, that's exactly what we
observe. Several of the new clonal
clusters that are appearing in this serotype 19A disease used to be, in fact,
associated with 70-valent conjugate vaccine types. So the really key message here is that previous vaccine serotype
strains have essentially switched their capsules to become 19A strains.
Well,
19A is clearly a problem, but are there also other serotypes that are causing
replacement disease in children, and that's what this slide shows. Serotypes 3, 15, 22F, 33F and 35 all have
increases in invasive disease among children under the age of 5. And for serotypes 3, 15 and 33F these
findings have been confirmed by other investigators using other data sources.
So
to summarize in children we've seen a dramatic reduction in the vaccine type
invasive disease among children under the age of 5 with a substantial indirect
effect among older children. There are
some concerning increases in non-vaccine type disease, especially 19A. And there's substantial evidence now for
capsular switching as a means of evading the vaccine induced immunity.
Now
let's go on and talk about adults. This
is a very similar slide to the first one I showed you in children, only this
breaks down adults into four different age groups. Those 18 to 49 in the green line at the very bottom. Those 50 to 64 years of age in yellow. The 65 to 79 year olds are in pink. And the white line at the top represents
adults 80 years of age and older.
So
on the left hand side it should be pretty obvious that the rates of disease
vary considerably by age group. And
notice that the population 80 years of age and older had a baseline rate in
1998 and '99 that was almost identical to the rate that we were seeing in
children under the age of 5. However, over the subsequent years rates of
disease in all of these age groups have declined substantially by about 20 to
40 percent and all of these changes are statistically significant.
So
let's ask the same question again: Is
this truly attributable to the vaccine?
And one way we can look at that is by looking at changes in vaccine
serotype disease.
These
are the rates of disease in adults caused by the seven serotypes in the
conjugate vaccine. And I think what's
pretty striking is how similar all of these declines are. No matter which age group you look at you
see anywhere between a 65 percent and a 75 percent reduction in invasive
disease caused by these vaccine serotypes.
These are all statistically significant changes, and obviously this has
all hurt immunity.
One
question that we often get a lot is how do you know that this is not
attributable to either consistent or increased use of the polysaccharide
vaccine? And one way to get at that
question is to look at those serotypes that are contained in the polysaccharide
vaccine but not in the 70-valent conjugate vaccine. And that's what this slide shows.
So
these are those 16 serotypes. And you can see from 1998 through 2004 there was
essentially no change in any of the age groups. If anything, there was a slight
increase in the rates of these 16 serotype invasive disease cases among persons
aged 50 to 64, which is shown in the yellow line.
So
the key message here is that we do not think that these overall declines in
invasive disease are related to polysaccharide vaccine. It's more likely that this is hurt immunity
from the conjugate vaccine.
What
about those vaccine related serotypes minus 19A? Remember that we saw substantial cross protection in children
under the age of 5. Probably no cross
protection in children 5 years of age and older, and that's a similar thing
that we're finding here. No statistically significant changes in the rates of
vaccine related disease minus 19A in the adult population. So really no indirect cross protection has
been observed in this population.
Getting
back to this same serotypes 19A question is it happening in adults? And the answer is a pretty resounding
yes. So between 1998 and 2004 we saw
increases of anywhere between 77 percent and 2010 percent among the different
age populations. All of these are statistically significant. Again, however, I
need to draw your attention to the Y axis.
Remember we were looking at rates of disease in the oldest age
population of about 100 cases per 100,000.
And now we're barely up to about eight cases per 100,000 in that same
group. So statistically significant and
relatively large increases in the instance of 19A disease, but in comparison to
the reduction in vaccine serotype disease, it's still comparatively small.
Non-vaccine
serotypes other than, this is actually including 19A and all of the other
ones. It seems that it's really
statistically significant in the age population of 50 to 64 years of age. What about other non-vaccine serotypes? 19A is obviously statistically significant,
but so in serotype 15, 33F and 35. So
19A is not the only story, but it is the majority of the replacement disease.
What
about trends in syndromes and comorbid conditions? I'll refer you to the paper cited at the bottom here by Katherine
Lexau that was published in JAMA a few weeks ago. She looked at a number of issues related to
invasive disease in adults 50 years of age and older. The two that are highlighted here are syndromes and comorbid conditions. Essentially we observed that the incidents
of meningitis was unchanged from 1998 to 2003, while bacteremia and invasive
pneumonia cases decreased substantially over that time period.
In
terms of comorbid conditions we saw that the proportion of case patients with
HIV, diabetes, COPD and immunosuppressive therapy all increased. Now, this
wasn't because the absolute rate of disease increased in those
populations. It's that the absolute
rate of disease in the healthier populations decreased so much. So as a proportion of the total these
individuals make up a larger proportion of our invasive disease cases.
We
also saw that the proportion of case patients with at least one indication for
the polysaccharide vaccine increased from about 62 percent to 72 percent.
Well
I mentioned that HIV was one of those underlying disease syndromes that was
becoming common in our case patients, and that's sort of what this slide is
getting at. On the top half of this
slide we're looking at rates of vaccine serotype disease among adults aged 18
to 64 of age with HIV or AIDS. In the
lower half of the slide we're looking at vaccine serotype disease in adults 18
to 64 years of age without HIV or AIDS. So all of the other populations
combined.
And
what you see here is a fairly consistent decrease of about 60 percent in the
rate of invasive disease in both of these populations. Now what about serotype
replacement? In the HIV/AIDS population
we actually saw a 43 percent increase in the rate of non-vaccine type serotype
disease, whereas we saw no statistically significant change in the rate of
non-vaccine serotype disease among persons 18 to 64 without HIV or AIDS.
I
would also point out that the rates here are remarkably different. The scale
for HIV and AIDS goes up to about 700 cases per 100,000 whereas for the lower
half of the slide it's about 10 cases.
What
about actual changes in mortality? This
slide is showing the mortality rate, actually both in children and in older
adults expressed as deaths per 100,000 population. In the baseline period of 1998 and 1999 the mortality rate from vaccine
serotype disease in children under the age of 5 was about 0.53 deaths per
100,000. And by 2004 that rate had declined by more than half to about .16.
For
non-vaccine type disease the rate increased a little but, from about .08 deaths
per 100,000 to .15. And overall, we still saw a substantial approximately 50
percent decline in the mortality rate for children.
Well,
what happens if we look at the same thing in adults? We saw a very modest decline in the mortality rate for adults 65
years and older for vaccine type disease.
A small increase for non-vaccine type disease. And the overall change is essentially zero. So sort of a disparity in the impact of the
vaccine on mortality rates.
So
to summarize the impact in adults, we saw a dramatic reduction in vaccine type
disease among adults aged 18 and over.
Some concerning increases in invasive disease caused by serotypes not in
the vaccine. And the remaining cases
are more likely to have comorbid conditions than several years ago.
To
try to put all of this in perspective because I've been talking direct and
indirect effects so much, this slide was published in the Morbidity and
Mortality Weekly Report back in September.
The bar on the left hand side of the screen shows the number of vaccine
type invasive disease cases prevented by direct immunization of children. And it was approximately 9,000. But notice
the bar on the right, which is the number of cases prevented among individuals
who are not targeted for the vaccine, so that would be older children and
adults. The indirect effect of this
vaccine has been roughly double that of the direct effect. I think many of us were hoping initially
that we would see some indirect effects. I don't think any of us expected that
it would be an effect of this magnitude.
What
about expected serotype coverage in adults for different vaccine
formulations? To reorient you, this is
not a slide showing rates of invasive disease over time, but the proportion of
all of our invasive cases that are caused by serotypes in different vaccine
formulations. So at the bottom in the pink line that represents the 7 serotypes
in the currently available conjugate vaccine. If a 9-valent vaccine were to
become available for adults 18 years of age and older, and if that vaccine
contained serotypes 1 and 5 in addition to the 7-valent serotypes, then we
would see the yellow line. So this is a
decline in a proportion of all invasive cases caused by those 9 serotypes over
time.
The
next line up, the green one, represents an 11-valent product which would
contain the same serotypes as the 9-valent product, plus serotypes 3 and 7F.
For
the 13-valent product indicated by the white line, this would be the same as
the 11-valent product except with 6A and 19A. We still see some declines, but
not merely as much. And you can
understand that now that we have pretty clear understanding of what's happening
with serotype 19A and 6A.
And
then finally at the top in the blue is the serotype coverage that we're seeing
over time for the polysaccharide vaccine.
Now you might ask, do these changes differ by age group? So now I'd like to just focus on calendar
year 2004 and break it out by different age populations.
So
in the 18 to 49 year old age group the pink bar represents the proportion of
all invasive disease cases caused by the serotypes in the 7-valent conjugate
vaccine. In 2004 that number was about 24 percent.
For
a 9-valent product it was about 26 percent.
For
an 11-valent vaccine, 35 percent. If
you then add in serotypes 6A and 19A, we go up to about 54 percent.
And
finally with the polysaccharide vaccine we're at about 84 percent.
These
changes are pretty consistent across all of the age groups, although there are
some minor variations within individual serotypes.
So
in summary, serotype coverage ranges from about 22 to 85 percent depending on
the vaccine and the age group. The 7
and 9-valent formulations are virtually equivalent in terms of their serotype
coverage. And the 11, 13 and 23 valent
vaccines would theoretically have incrementally more coverage from about 35
percent to about 85 percent.
Finally,
what about opportunities for evaluation of new vaccines in adults. In the
absence of a controlled trial what could we at CDC potentially do to help with
this issue? One possibility is to do
post-marketing surveillance for invasive disease. In fact, as long as we have
the support to do it, we will continue to do surveillance for invasive disease
in all age groups. This, however, could
also curve through other, perhaps, administrative systems such as Medicare. I
think a fundamental concern about that is that there's generally no serotype
information in those databases and, as Dr. Pratt indicated earlier, there are
some issues around specificity.
Regardless
of whether we look at ABC's data and administrative databases, we're also sort
of looking at ecologic or temporal relationships. And that always makes it more difficult to assign causality
despite everything we can do to look at individual serotypes or collections of
serotypes.
Finally,
we could do a case control study to evaluate the effective of conjugate vaccine
in adults. This is a very reliable
method that's been used for many years. There is some very recent experience in
conducting such a study in children.
We
could adjust for the routine use of polysaccharide vaccine. The major downside is that this would be
quite expensive and very labor intensive.
So
with that, I'd like to acknowledge all of the collaborators who participated in
ABCs.
And
thank you for your interest.
CHAIR
OVERTURF: These three papers are open
for questions and discussion. Are there
questions or comments from the Committee members? Dr. Markovitz?
MEMBER
MARKOVITZ: Just so I understand this
rather key point. I know this was
addressed, but I'd just like to hear a little bit more.
In
terms of the opsonophagocytic assay there's no -- well, even though it's well
validated in the lab, it's not validated yet as a measure of true immunity in
patients, is that correct? Certainly
not in the elderly. And it wasn't clear
about what the story is with younger people.
Could someone speak to that, since that seems to be a central issue
here?
CHAIR
OVERTURF: Please identify yourself,
DR.
STEINER: Yes. This is Dr. Sandy Steiner, CDC.
And
I believe you are correct. It hasn't been validated at that point. So those studies will have to be put forward
before you can use it that widely, I imagine.
MEMBER
MARKOVITZ: Short of a very large
clinical trial with that as a component of the trial, how do you think this
could be validated? Is there a way to
validate it in a more brief way or something like that.
DR.
STEINER: The validation has been only
for infants. And because we are
discussing here is the adult vaccination, we have to concentrate on the adult
population. And so it should be part of
a clinical component trial of a large efficacy trial for adults. And the Finns included these as one of the
components when they were trying to the titers measurements and trying to validate
for titers. And they also salivary
measurements and they looked at all the components too when they were trying to
evaluate other endpoints that will be maybe protein candidates and everything
like that.
So
I think that in that respect you should consider it as part of the efficacy
trials.
MEMBER
MARKOVITZ: Perhaps you said this and I
missed it, but how good are the data correlating this assay with the
protections seen in the infants? Was
that part of the original trial or --
DR.
STEINER: These was a subcomponent of
the study, that's my understanding.
That the black Northern California KaiserPermanente had its own endpoint
and that only a subset of sera was evaluated for opsonophagocytosis. And that's what was published in the Judar
paper where it was laid out available for a subcomponent of those sera that
were posed those three for infants. And
that's the only data that I have right now where there is a direct correlation.
There
are data also from the clinical trials that the Finns have done. And they will also see correlation between
opsonophagocytosis and ELISA and their protective levels. So all those trials
are also available and in the literature.
If
we put all the trials together, I think you will have enough information to put
more weight to what opsonophagocytosis can do.
That's a measure.
CHAIR
OVERTURF: I think Dr. Self had a question.
MEMBER
SELF: Yes. I'm interested in the
serotype replacement question. First I
thought the presentation of the data from the ABC was really terrific.
So
you pointed out that the increases that you see up to 2004 are small in
absolute magnitude. But I also couldn't help but have this feeling that the
shape of that curve looked like the beginnings of an expediential kind of
curve. And I'm thinking about the drop
in all of the other vaccine related serotypes as creating this vacuum into
which these 19A and perhaps others will be drawn.
Have
you done any modeling work or would you hazard any prediction about over the
next couple of years where those replacement serotypes are going to go?
DR.
MOORE: The short is answer is no, we
haven't. We would be very interested in
doing that.
One
thing that might help a little bit in that regard is to ask the question well
why 19A? You know, why not something
else? And I think the answer is a two
part answer.
First
of all, serotype 19A was already quite common before the 7-valent vaccine was
introduced.
Secondly,
it was already more likely to be antibiotic resistent than some other vaccine
serotypes. Excuse me. Than some other non-vaccine serotypes. So in that sense 19A was sort of waiting at
the door and it had this survival -- actually two survival advantages of being
more likely to be antibiotic resistance and not already covered by the
vaccine So in terms of looking forward,
we could try to figure out what are the next serotypes that are waiting at the
doorstep, so to speak.
DR.
STEINER: I would like to add a comment
to that, too. And it is regarding the
thought that there will be some cross protection between -- if you include 19F
in the vaccine that you will cross protected to 19A. And as you can see, there is evidence for the cross protection
not to be present. And that is very
important because in function when you're measuring the function and you look
at type specific antibodies and only if it's type 19F as a target will you be
able to have good functional antibody activity.
So
this adds information about functional antibody activity . We should not assume that we're going to
have function that is cross protected.
We have unpublished information for serotypes 15B and C which differ
just by the -- of the polysaccharide and there is no cross protection of
antibodies that are to 15B with functional antibody activity to 15C. And the only difference is the -- in the
polysaccharide. The structure is exactly the same for the two.
CHAIR
OVERTURF: Dr. Piantadosi?
DR.
PIANTADOSI: Thank you.
I'd
like to return just for a moment to this question about OPA and its role as a
potential surrogate. I understand that it hasn't been validated in adults as a
surrogate outcome. My question is if it
were validated in adults for a particular type of vaccine, is there evidence
that it would then also be valid as a surrogate for other types of vaccines?
DR.
STEINER: You mean other conjugant
vaccines or other vaccines outside of pneumococcus?
DR.
PIANTADOSI: No, no. Other conjugates or other approaches to
vaccines?
DR.
STEINER: Like polysaccharide vaccines?
DR.
PIANTADOSI: Yes, exactly.
DR.
STEINER: Okay. When we have conjugate vaccination it's type
specific antibodies being generated. So
we can assume that protection will be applicable as a correlate of protection
to the conjugate vaccines that are coming up.
But when it is protein vaccines, you will not be able to use the same
surrogate because we don't know all the mechanisms for function for each of the
protein candidates that are being proposed.
Some
proteins will mediate colonization, others may interfere with invasion. And the mechanisms by which they act or
function may be totally different. Some
of them may have opsonophagocytic activity and there are products that are
being evaluated in that manner. But not all the products will have these
opsonophagocytic activity. They may
have a different functional antibody measurement that is needed to be able to
evaluate them.
CHAIR
OVERTURF: Yes. Dr. Hetherington?
DR.
HETHERINGTON: There are a number of
questions that use of OPA raise with regard to use of the surrogate
marker. We haven't talked about the
pathophysiology of invasive pneumococcal disease. For infants it can be primarily a bacteremic disease and so it
may make some sense to talk about serum titers and the use of utraphos. But what about for pneumonia? And it raises two questions.
Would
studies utilizing pulmonary secretions be more appropriate. And what do we know about the transfer of antibody raised by vaccines across
mucosal surfaces and its presence in pulmonary secretions?
DR.
STEINER: Well, that's a very difficult
question. And, yes, most of the
studies that have been done has been assessing the serum antibodies.
Mucosal
antibodies have been looked at by the Finnish group and they've looked at
introitus trials. And so there they
could probably, if you review those, you will be able to see the correlation
with protection. But the transportation
of antibodies from the serum at the minimum levels that are needed in the
mucosal surface to prevent, for example, colonization are also unknown. And there have been studies for hemophilus
and influenza but for pneumococcal they haven't done.
For
invasive disease like pneumonia as an endpoint it's even harder because we're
having a hard time even defining pneumonia and the endpoints in the trials. The
antibodies that will protect against pneumonia and with the background it's
even harder to decide what will be the minimum level. Diagnoses of pneumonia
and differentiating viral pneumonia and different etiologies of pneumonia, it's
a major factor before we can even correlate to our laboratory correlated
protection.
CHAIR
OVERTURF: I'd like to ask Dr. Moore
before he leaves, you mentioned the possibility of case control trials as a
mechanism. What would be the
possibility and the logistics of trying to combine a case control trial with an
evaluation with opsonophagocytic assays?
It seems to me although it would be labor intensive, it might be one of
the quickest ways to get some of this answered.
DR.
MOORE: I think the biggest barrier
would that our surveillance program is really based on -- it's an observational
program. So patients are admitted to the hospital or seen in outpatient
clinics. They're diagnosed with
invasive pneumococcal disease. And then
that case report and that isolate comes in days, weeks, months later depending
on the situation. Because it is often very difficult to collect all of the
information that's needed for the case report from.
So
I think it's an issue of timeliness that you would want -- I presume you would
want information about OPA early on at the time a person is diagnosed. And we
typically do not collect serum, for example, at the time a person is admitted
to the hospital and becomes a part of the surveillance program.
CHAIR
OVERTURF: Do we know anything about
what happens to the OPA titer during acute pneumococcal disease? That was always an issue with the antibody
studies because there was always a concern about decreases, actually, in antibody transiently?
DR.
STEINER: Yes. Actually there is -- this
probably has not been published either, but there is information regarding
C-reactive protein. And in acute phase you will circulating C-reactive protein
and that will effect opsonophagocytic titer.
So when you do your absorptions of your sera you should dilute the sera
to a higher initial dilatation to be able to dilute out the C-reactive protein
and also measure the background of the C-reactive protein. I think this is very
important to consider because it could enhance the opsonophagocytic activity --
so that is factor.
CHAIR
OVERTURF: I think Dr. Farley was first.
MEMBER
FARLEY: Mine is more based on the
epidemiology. In some respects the
initiation of the conjugate vaccine in infants has probably been more effective
in preventing disease in adults than the polysaccharide vaccine that's been
around for a long time. And so I guess
as we look at in the introduction or the process of introducing a conjugate
vaccine in adults I'm wondering what we can add and how we should approach it. And another way is should we be looking at
what the infant vaccine hasn't done and fill in the gaps in the adult
vaccine. And that brings 19A right to
the forefront and wondering if that should be fairly high priority for any
conjugate vaccine in adults is to include that, or considering modifying a
pediatric vaccine I guess would be another approach. But looking at the replacement or the prominent ones in a era of
fairly good immunization of infants with this conjugate vaccine and looking at
how we can work together in that system in the U.S., and I don't know if you
have any comments on that.
DR.
MOORE: Just that I would totally agree
with Dr. Farley on that. I think it
would be hard to envision how we would get a control on invasive disease in adults
without something that would be effective against 19A since that seems to be
the prominent one now. Obviously,
including some of those serotypes would be helpful as well.
CHAIR
OVERTURF: Dr. Royal?
MEMBER
ROYAL: First of all, I'd like to say
that Dr. Steiner and others are to be commended on the work that they've done
in development and validating the opsonophagocytic assay. But you would think that the more reasonable
way to go would be instead of using an assay that uses HL60s, which aren't even
mature neutrophils would be to use the patient's own neutrophils in a sort of
modified ELISA assay.
DR.
STEINER: Well, the only spot assay
actually only looks at the B-cells that are producing the antibodies. So you will need to work with PAFI codes.
And to truly have a good estimate of what are the cells that are producing the
antibodies you should really have bone marrow samples or something like that,
it's impossible to do. But if you're
working with peripheral blood, you will only work with the PAFI codes.
If
you wanted to use the own host phagocytic cells, there have been reports in the
literature that were cautioned a little bit about the function of the
antibodies as people get older. And because the target population of the trials
will have to be considered, the ages.
Most of the trials that are being done or the studies that are being
done are with really young elderly.
People that are only 65 years or 70 or so. And really function starts going down as we get really, really
old like 80, 90 years of age.
And
with age there has also been the concern about the phagocytic function of the
cells also not be as efficient in carrying out the function. So if you used the own host cells, you could
take them but you'll need to have -- you'll have two parameters there. One, the
function of the host at the time and the other one will be do they have
antibodies circulating at the time, that will be need to observed out. And the
other question that you have is the variability between the receptor's other
phagocytic cells because there are differences in the receptors from donor to
donor. Some of them are not
significantly higher finity to the various immunoglobulins that they complement
as if you use one single standardized.
So
if we want to compare across, it's probably easier to use for being able to
compare one vaccine another vaccine in one population against another
population across ages, a standardization is an absolutely necessity under
those conditions.
CHAIR
OVERTURF: Dr. LaRussa?
MEMBER
LaRUSSA: Well, I'd like to expand on
that answer a little bit. And I would
argue that what you need are age match controls depending on the population
you're looking at. Because you're going
to come up with a level of antibody in a certain population, probably children
or young adults, that correlates with the functional correlate, which is
phagocytic activity. And then use that level of antibody as a target to get for
the elderly population. And it may not work.
You may need age match phagocytes in your study to see what the level of
antibody you need in the elderly is.
DR.
STEINER: Well, we have two components.
One is the phagocytic cell, which is a question on it sown. And the other one
of the antibodies that are induced by the vaccine. So the major question is the function of the antibodies induced
by the vaccine. The secondary question
is the function of the phagocytic cell in the host that can vary by many, many
parameters. Whatever, you know,
compromising conditions they may have or by age.
CHAIR
OVERTURF: Dr. Karron?
MEMBER
LaRUSSA: But I guess if you're looking
for a correlate of protection in the elderly, then you have to look at the
second component, too. You can't just
look at the antibody.
DR.
MOORE: Exactly. That's my point.
DR.
STEINER: I think the studies need to be
designed to have that in mind as one of the items that needs to be looked at
functioning in the host. Yes, I don't
think that that can be ignored. It just
has to be addressed, but maybe on a separate type of study.
CHAIR
OVERTURF: Dr. Karron?
MEMBER
KARRON: Actually, I have one question
for Dr. Romaro and one for Dr.
Moore. So my question for Dr. Romaro is
just to set back for a second. For the
OPA assay in any system, in animals, in children, anywhere, has it ever been
shown to correlate with protection against pneumonia.
DR.
STEINER: No, we already answered this
question.
MEMBER
KARRON: No. I didn't think so, but I just wanted to be clear on that.
DR.
STEINER: Yes.
MEMBER
KARRON: And then my question for Dr.
Moore is can you say something about serotypes and antibiotic resistance
currently?
DR.
MOORE: If I can have my slides back I
can. I think it would be substantially
easier to show that to you than to try to explain it.
Yes,
I didn't think I would have time to discuss this during my talk so I brought
these as extras.
This
slide, it's a bar chart showing the most common current serotypes in adults in
2004. So this is all adults 18 years of age and over ordered in decreasing order
of frequency. So 19A is most common
right now. 22F, 4, 3, 6A, etcetera.
The
height of the bars themselves just represent the total number of cases we have
caused by these serotypes.
The
red portion of the bar represents the proportion of those serotypes that are
not susceptible to pneumonia. So
overall if you lump at all of these streams together, we're looking at about 20
percent non-susceptibility to penicillin.
That gets back to this question of why 19A. It was already common and it
was already antibiotic resistent before introduction of the vaccine. And we're seeing that those survival
advantages are still holding it around.
The
next one in line of terms of antibiotic resistance for penicillin would
probably be 6A. But overall, these replacement
serotypes appear to be less resistent than the initial ones.
Similar
slide for erythromycin shows that the overall rate is very similar, about 18
percent. It's just that we see a little
bit of resistance and lots of different serotypes instead of having all the
resistance focused in one or two serotypes.
CHAIR
OVERTURF: Dr. Self?
MEMBER
SELF: I just want to close the loop a
bit on the issue of study design. Case
control studies can be just fine for estimating efficacy. But retrospective
studies don't work very well, if at all, to assess correlates. The only possibility there is if you can do
the assays on storage specimens and you have specimens that are prediagnostic.
And none of that, I think from my understanding, is true in this case.
So
if we're looking at evaluating a correlate, we are talking about prospective
studies with specimens collected in some sort of regular fashion.
CHAIR
OVERTURF: We need to break for lunch at
this lunch. There will be ample time for more discussion for the afternoon.
So
we'll break at this time and reconvene again promptly at 1:00.
(Whereupon,
at 12:06 p.m. the meeting was adjourned, to reconvene this same day at 1:06
p.m.
A-F-T-E-R-N-O-O-N S-E-S-S-I-O-N
1:06
p.m.
CHAIR
OVERTURF: I'd like to call the
afternoon session to order.
The
first item on the agenda is the open public hearing. So I'll turn the meeting over to Christine.
SECRETARY
WALSH: Good afternoon.
As
part of the FDA Advisory Committee meeting procedure we are required to hold an
open public hearing for those members of the public who are not on the agenda
and would like to make a statement concerning matters pending before the
Committee.
I
have no received any requests at this time.
Is there anyone in the room who would like to address the Committee at
this time?
Dr.
Overturf, I see no response. I turn the
meeting back over to you.
CHAIR
OVERTURF: The first presentation of the
afternoon is Jan Poolman who will speak for GlaxoSmithKline.
PARTICIPANT: I'm sorry.
I'm going to go get him. He's upstairs.
Just a minute.
(Whereupon,
at 1:09 p.m. a recess until 1:11 p.m.)
DR.
POOLMAN: Can I start?
Well,
I apologize. But my paper said it was
starting at half past 1:00, so I just busy with some other things. Sorry about
it.
And
thank you very much for invitation to speak on pneumococcal vaccines, which I'm
doing with great pleasure.
At
GSK Biologicals we have an intensive program pneumococcal vaccine development
and we in late stages of development of a pediatric 10-valent conjugate
vaccine. And we're also highly
committed to develop an adult pneumococcal vaccine.
You
may not know, but int he past GSK Biologicals, which was named differently in
those days, developed a 17-valent vaccine when it was finally decided to stop
and not continue to 23. And so all the
experiences there and we are planning to build on our experience with pediatric
conjugate development to develop adult vaccines, which are for the shorter term,
focusing on conjugate vaccines because of polysaccharide immunity, all well
know, but also for the longer term we have programs on pneumococcal proteins,
although the ideal scenario for a common antigen is obvious, but it's also
obvious that is of a scientifically high risk because much less is known.
So,
I will speak only about polysaccharides and conjugates in this presentation.
The
situation with respect to polysaccharide immunization is that the current
situation does give a substantial public health benefit by using the existing
23-valent polysaccharide vaccine, most by impacting on bacteremia, pneumococcal
bacteremia.
It
is somewhat contrasting but despite the substantial public health benefit the
vaccine and its use have actually a marginal impact on the total burden of the
disease, which if you add the two together would mean if you have a good
program, you would have really an impressive impact on the burden of
pneumococcal disease.
The
reasons for the marginal impact are that the vaccine is only given once and
also because the impact on pneumonia is shown to be low, although the actual
level of protection against pneumonia is unknown.
So
what are the reasons? And it has been
demonstrated that the polysaccharide vaccine has intermediate efficacy against
bacteremia. Most of these cases
associated with what I call here about 50 percent efficacy are related to
bacteremia. And like I mentioned,
there's low efficacy against pneumonia.
The precise level is unknown due to underpowering of the studies, but
certainly also because of the difficulty to diagnose.
These
data do suggest, and I'll come back to that later as well, in the pediatric
context that it is easier to prevent bacteremia as compared to pneumonia.
One
other major limitation of the existing situation is that the polysaccharide
vaccine is only given once. There's no
policy of revaccination. And this has a
relationship with the uncertainty of lowered responses upon revaccination,
which we also call hyporesponsive. I
call it uncertainty and I will mention one slide, and then I will stop talking
about hyporesponsiveness and focus on the polysaccharide immune responses.
Here I put a quote from a not to long ago review
on revaccination. And I think this is a
fair statement. The limited data
indicate that the responses upon the second dose are lower and the number of
factors could play role, but definitely also the initial vaccination itself
could play a role in these lowered responses.
So
there is a need for further data here, particularly also looking at individuals
that by themselves have a low response upon the first immunization, which is
well known for any polysaccharide vaccine, even in pediatric, but also in
adults with other polysaccharide vaccines, any polysaccharide vaccine does not
completely immunize all subjects. There
is a substantial portion, a minority but there is a substantial portion of
individuals that respond poorly to a polysaccharide. In general, with conjugate vaccines that poor response is
resolved. This the data with other
types of conjugate vaccines.
And
it may very well be that revaccination of these already poorly responding
individuals get even worse and those type of data are highly needed, but yet
not yet known, but may play a major role in the limitations of the
polysaccharide vaccine.
So
now I go back to the polysaccharide immunity.
Here is just an illustration of what I mentioned. There is about
intermediate, I would call it 50 percent efficacy, against pneumococcal
bacteremia. And this the review of
Fedson and Musher in the Standard Book on Vaccines by Stanley
Plotkin. And it's a summary of many
studies. So it is intermediate, it's not complete.
This
is what I mentioned in my introductory slide. This results into a relatively
marginal impact on total burden of pneumococcal disease. So here I depict invasive disease, mostly
bacteremia and pneumonia. It's a
logarithmic scale, so it's a substantial difference. Much more pneumonia than
bacteremia. And this is what we
currently do. We give one immunization
at 65. That's what we understand from
it works for about five years. And it
works partially against bacteremia. So
approximately 50 percent. So you take
this piece of the burden of disease away while this all remains and it starts
rising, as you can see here. So already
way before 65. So this is a substantial
public health benefit, but it is a marginal impact on the total burden of
disease.
So
initially it was expected with the earlier data with the polysaccharide vaccine
that it would also be a significant impact on pneumonia. That was the expectation. And the expectations were driven by the
early data in younger adults, which actually showed quite decent efficacy
against pneumonia. And if you look
through these publication, it's clearly pneumonia and it's also clearly
non-bacteremic pneumonia.
There
is an impact with the polysaccharide vaccine on adult pneumonia. And the expectations after these studies
which led to the licensure of the vaccine were high. Then after licensure the vaccine got used in the older age. And the results have been rather
disappointing. Although, like I stated, the real extent is unknown because of
the lack of the power of the studies that were done and because diagnostic
tools were in general not sensitive enough.
So
why is the impact of the polysaccharide vaccine different in young adults than
elderly with relation to pneumonia.
There are a couple of explanations.
The antibody level is one. And
certainly they could be lower, although the data in the literature did not
suggest that there is a substantial difference. And I will show you some data also.
Then
functional activity. There are some
data out there, and I will show some additional data that confirmed these
earlier data. And that could be an
impact on functional activity.
Then
also the mediator of functional activity, the primary mediator of the
functional activity, the polymorphonuclear activity could be impacted as
well. So if I may forget to say it
further on, I think with what we need to do is with the current existing assays
that we use with cell lines, which are appropriate because they are robust and
you can validate them and use them in high throughput, but these need to be
validated in pilot studies and compared to -- from older adults, the elderly. Those kind of studies have not yet been
done. In my mind these need to be done.
Not to use them as a primary readout because that's not feasible, not
practicable, not robust. These assays
cannot be validated to the level needed. But to compare it to the assays with
the cell line.
So
antibody levels. You've seen this slide before. What we know from antibody levels and prevention of invasive
disease, mainly bacteremia in infants, is that you need low levels of
antibodies. And this was the result
from a WHO meeting, but it was based on the KaiserPermanente efficacy
data. You need low levels of antibodies
to prevent pediatric bacteremia.
This
is data that we have generated recently after polysaccharide vaccination in
above 65 years old subjects. And using
the highly specific assay that currently has become the standard for looking at
polysaccharide human responses for the pneumococcus, which includes both
intermission with polysaccharide and
22F polysaccharide. So finally after
decades of some confusion of assays against pneumococcal polysaccharides we
have an assay in hand that gives you the needed sensitivity and specificity
which has been lacking for long.
By
using this assay and using the similar principle was used for looking at what
are thresholds linked to the observed efficacy in the elderly, what you see
there is, what I mentioned, 50 percent efficacy against bacteremia mostly. And if you then look at 50 percent of
subjects immunized what type of level they would achieve, it's about 5 micron
per mil.
If
you would look at the difference, the delta between the two, you come a little
bit lower. In the range of 2 or 3 micron per mil that differentiates the best
between the non-immunized and the immunized. But the bottom line message what
I'm giving here, you need approximately ten times more antibodies in the
elderly as measured ELISA as compared to pediatric to prevent pneumococcal
bacteremia. Now why is that?
And
I come back in a conclusion slide yet right after this. And here is a great
part of the explanation. Is we looked
at immune responses in young adults, 18 to 25 mean age 30 years, and in elderly
subjects above 65 mean age 72 immunized with the existing polysaccharide
vaccine and we looked against the antibodies determined in ELISA as shown
here. Not much difference. This is in
line what has been shown in literature.
There is significant differences.
If
you would do an aggregate analysis there's approximately twofold
difference. However, if you start
looking at opsonophagocytic activity, the differences become huge, really
dramatic, I would say. And you see most
of them are significant. If we had used a little bit higher numbers, all of
them would have been significant. And if you would do an aggregate analysis
there is approximately five fold difference.
Now,
I just mentioned that if you look to the antibodies levels needed to prevent
bacteremia there was about a ten fold difference. And here with opsonophagocytic activity between young adults and
the elderly, you already find a five fold difference.
So
if I go back to what I postulated here, certainly this is one of the key
explanations of this question. It is a substantial of the answer.
So,
like I mentioned, you need a much higher anti-polysaccharide antibody levels in
the elderly to prevent bacteremia as compared to young children. And which can be explained in a number of
ways, but certainly like I mentioned decreased opsonophagocytic antibody levels
is a major player. And like I
mentioned, we do need to look at PMN functionality in the elderly as compared
to the cell line that we are using. It may give some additional explanation.
These
are general also explanations that can play a role. Bacteremia in adults are mostly associated with pneumonia. They are not in children. And the responses to polysaccharides could
in general be of less quality as compared to conjugates. Although in young adults that doesn't seem
to be really an outstanding observation.
So
how does all this translate into the observation that, indeed, it is possible
to prevent pneumococcal pneumonia. I've
mostly talked about bacteremia now, but how does that translate into the
observations made on pneumonia?
Like
I showed earlier, the earlier trials in young adults did show that the
polysaccharide had a clear impact on pneumonia in young adults, substantial
impact. It has been shown that conjugate vaccines have had a substantial impact
on pediatric pneumonia. It is possible.
And the fact is that observations in the elderly are the exception.
Those are the outlier. And I just gave
I think a quite reasonable explanation which explains for a great proportion
the reason why that is, why in the elderly do these existing vaccines prevent
pneumonia so poorly.
And
I've heard some discussion this morning on what is the mechanism of protection
against pneumonia. And there was a
suggestion that there's not much evidence of that -- opposite the facts killing
with PMNs play a role. I would like to turn that around. What other ways to explain it? These are intermuscular immunization leading
to serum antibodies that do transudate.
And if you look to pathohistological observations for pneumococcal
pneumonia in the pre-antibiotic era, I think there is little doubt that only
after the appearance of PMNs at the site of infection there was the start of
signs of cure. And if you ask for 100
percent proof, definitive proof, that is difficult to give, never to give. But
to put it on the other side that there is no evidence that what is the
mechanism of protection here, I would say that is putting it in a situation
which I think is highly unlikely. I
really do think that antibodies that you induce by systemic immunization and in
associating with polymorphonuclear sites are the primary mechanism of
protection.
So
this is just to illustrate the data that it is possible to prevent
pneumonia. Here are the data with a
9-valent conjugate vaccine in South Africa and Gambia. It also shows a tendency that it is easier
to prevent invasive disease, mostly bacteremia, as compared to pneumonia. Its point estimates overlapping confidence
intervals, but usually point estimates point you in the right direction. And it is in the same line what is observed
in the elderly with polysaccharide vaccine.
And
interestingly, the studies in the Gambia did not show a difference, again
accepted widely overlapping confidence involved, but they did not show evidence
of a difference in bacteremia or non-bacteremia pneumonia. I think also confirming the earlier trials
in young adults with plain polysaccharide vaccine.
So
I do think it's fair to state that it is easier to prevent bacteremia, but it
is certainly possible to prevent pneumonia.
So
how do we achieve the situation that the exceptional situation in the elderly
where you have a poor impact on pneumonia can be improved? Well, one of the primary one is the
anti-polysaccharide response needs to be made stronger, needs to improve
because there is definitely a link between antibodies and protection. And you need higher antibodies levels, more
functional antibodies also to improve the situation on bacteremia because 50
percent prevention of bacteremia is not satisfactory, even if you have a
23-valent coverage, if you have 50 percent protection you have, let's say, an
11-valent vaccine. And that is
certainly also needs, a high level of antibodies, against the polysaccharide
for more morphonuclear antibodies to start to expect and to realize an impact
on pneumonia in the elderly target population.
Higher
antibody levels are needed. More
functional antibodies are needed.
And
also the broadening of the immunization just beyond the one immunization at 65
is needed. And in order to do that you
need to be sure that revaccination is not leading to lower the responses. Like I said, we need more data to clarify
the situation, but I do think it is very suggestive what has happened in a
number of situations, not only with pneumococcal polysaccharides, but
pneumococcal polysaccharides particularly in the ones that respond poorly in
the first side will lead to even responses after a second immunization.
We
need more data, but it certainly needs to be resolved. And there indications that with conjugate
vaccines this can lead to a better situation.
So
I will end with a conclusion slide that what does this mean licensure of new
vaccines. And which logically are, as
you can hear from the presentation, are pneumococcal polysaccharide protein
conjugate vaccines. And they do have
the potential to improve.
I
think my colleague from Wyeth, George Siber, will in his presentation
demonstrate that it is possible to improve upon polysaccharide with
conjugates. So in that context, what
are licensure criteria for conjugate vaccines?
Immunonon-inferiority
against the polysaccharide responses in the elderly or in similar age groups to
my mind do need to lead to licensure acceptance for invasive disease or
bacteremia. It's a similar approach we
have been using for conjugate vaccines in pediatric. It's a similar approach we have been using for conjugative
vaccines in teenagers against meningococci.
I see a little doubt in this area.
Then
there is another interesting one which you could kind of hear during my
presentation. What if you achieve with a new polysaccharide vaccine a conjugate
vaccine? If you immunize elderly how
would you feel about these data if you reach similar antibody levels, similar
functional antibody activity as compared to what the existing polysaccharide
vaccine has done in young adults, which certainly the current vaccine is not able
to do? But what if your new vaccine would be able to do that and you know these
data that exist with the polysaccharide vaccine in young adults?
In
our view that is a clear steps towards expecting an impact on pneumococcal
pneumonia. And that is also a clear
step towards licensure for the pneumonia indication.
And
then finally, the response after revaccination need to be non-inferior
minimally, non-inferior to the response after the primary vaccination so that
there are no lowered responses. And in
particular in these subjects that are fully responsive from the first start
because those are the ones that are at highest risk.
So
here I would like to stop my presentation.
Thank you.
CHAIR
OVERTURF: Dr. LaRussa?
MEMBER
LaRUSSA: So two questions. One about the hyporesponsiveness after the
second dose. What we've seen mostly is
aggregate data. Have you separated out,
is there a subject of adults who are hyporesponders and could you look at
whether that's a function of their prior antibody titer? Maybe that's a subset that really can't
respond to polysaccharide antigens.
DR.
POOLMAN: It's a very good
question. And we will be able to answer
your question in I think about two years from now. What we have started to do, we have started to immunize a
substantial sample size of the elderly above 65 with the plain
polysaccharide. And with such a number
that allows us to separate them into response categories and then do a
follow-up study a couple of years later by comparing the polysaccharide and
then really have a clear view per serotypes, per response category of what is
happening with the second dose of polysaccharide. But we also intend in that study to compare it to conjugate
immunization.
So
we have decided to generate this cohort to give specific answers for specific
surrogates and for specific subgroups of poor, medium and high responders. It's
an ongoing study.
MEMBER
LaRUSSA: Okay. So the second question is in the slide that
you showed with the responses in the elderly where you had the two curves, the
pre-immunization and the post-immunization. And you said that what you did
there was you looked at approximately 50 percent efficacy in the elderly, which
was mostly you said in bacteremia. And
looked at what the antibody titer at 50 percent would be.
Now,
I know you don't have enough data to talk about efficacy against
pneumonia. But couldn't you separate
out the people who did and did not get pneumonia and look at what their
antibody titers were, and also look at them by the opsonic assay?
DR.
POOLMAN: Someone may want to comment,
but to my knowledge there is no data existing where we have baseline antibody
levels that can specific serotypes linked to their susceptibility to specific
serotypes pneumococcal pneumonia.
We
are in an ongoing study with our college from Sweden to look in some cohorts he
has. And it looks not unexpectedly that
we need to generate and analyze the data further, that there is a specific
deficiency in the anti-polysaccharide level or responsiveness in subjects that
later developed that specific type serotypes pneumonia, which all makes
sense. But we have rather limited data
in that respect.
But
I do strongly believe it's very specific event that the individual subjects
that are poor response or have low levels and that become colonized, other ones
that will develop type specific disease.
CHAIR
OVERTURF: We have time for only one ore
question.
DR.
JACKSON: Okay. Well, you've made the case that the
situation that we're contemplating about requirements for licensure of a new
conjugate vaccine in adults is similar to situations that have been encountered
in the past with meningococcal conjugate and with new Hib conjugates. But the
key differences that in those cases the new vaccine had at least equal disease
coverage as the old vaccine. And so if
you prove non-inferiority, that meant that the new vaccine was likely, at least
as good as the other one.
I
mean, here we're talking 11 serotypes versus 23. So it would seem to me that
even if you established non-inferiority for the 11 serotypes that the person
would still be at higher risk of disease potentially by not having the total
serotypes coverage. So I wondered if
you could address that concern?
DR.
POOLMAN: No, I fully agree with
you. The non-inferiority criteria is a
standard technical licensure criteria for which you have the guarantee that the
serotypes in your new vaccine are at least equal to the same serotypes in the
existing vaccine.
The
next discussion is, and I hinted to that like functional antibody activity as
well as hyporesponsiveness, that is a discussion that needs to develop what are
the -- I hardly dare to call them, but it's what you would probably have to
call them -- what the superiority criteria that you would need to see.
I
do think that if you show significant higher antibody levels, that that does
mean a stronger impact on the pneumococcal infection. And I do think that the absence of hyporesponsiveness if we
demonstrate will allow you to come with revaccination programs which are
currently not in place.
So
the non-inferiority criteria is the minimum necessary to tell you that the
serotypes in your new vaccine are at least equal.
DR.
JACKSON: I would agree. But in the absence of a correlated
protection I don't know what interpretation we can give to more. We can say at least equal, but if you say
twice as much -- I don't know that we know what that means.
DR.
POOLMAN: Like I said, that's a
discussion that needs to develop. But if you have clear superiority with
respect with respect to functional activity and you have clear difference in
superiority with respect to avoidance of hyporesponsiveness, I think that would
have to be taken into a consideration, into account. And ideally, it would lead
to a situation which I illustrated, that you would induce immune responses in
the elderly that are comparable to the adult situation with the existing
polysaccharide vaccine, which has clearly demonstrated a strongly impact in
that age group.
CHAIR
OVERTURF: We're going to have to
continue on because we're going to be short of time at the other end.
So
I'd like to call on Dr. Siber and thank Dr. Poolman for his presentation. Thank
you.
DR.
SIBER: Mr. Chairman, members of the
Committee, my name is George Siber. I'm
with Wyeth Life Vaccines. And I want to
describe for you a proposal for how a pneumococcal vaccine for adults can be
licensed.
What
I'll show you, what I'll discuss, is why there is a need for another
pneumococcal vaccine in adults.
Secondly,
the advantages of the conjugate pneumococcal vaccine for adults.
Third,
the potential public health impact of such a conjugate vaccine in adults.
The
proposed regulatory basis for licensing such a conjugate.
And
finally, some discussion of the feasibility of performing clinical efficacy
studies or lack of feasibility performing clinical efficacy studies with an
adult conjugate vaccine.
So
the first question is why do we need another pneumococcal vaccine for
adults? Well, because there are limitations. They've already been discussed by the other
speakers of the 23-valent polysaccharide vaccine. Antibody titers and efficacy appear to wane after 5 years. Effectiveness is very low in the
immunocompromised patients. 23-valent
polysaccharide induces hyporesponsiveness to either another dose of 23-valent
polysaccharide vaccine given later or to a dose of conjugate vaccine, which
I'll show you shortly.
Revaccinations
cause more severe adverse events. And
multiple authors have described that.
And therefore, as a general rule 23-valent is given only once which provides only a narrow window of
protection during a prolonged period of risk beginning at about 50 years of age
and increasing as we saw this morning progressively with advancing age.
And
the second reason is because there remains a substantial burden of invasive
pneumococcal disease in the U.S. These
are 2004 rates here. With the impact of
herd immunity already recognized from childhood -- and with 60 percent uptake
approximately of polysaccharide vaccine and despite that as you see here in the
older age groups there are still substantial rates of pneumococcal invasive
disease and substantial number of deaths in the older age groups especially.
The
second question is: What are the advantages
of a pneumococcal conjugate vaccine for adults?
The
benefits of a conjugate over polysaccharides in this age group, and I'll show
you the data to support the statements I'm going to make here, are the
conjugate antibody responses are significantly better or non-inferior to
23-valent polysaccharide vaccine by both ELISA and by OPA measurements. Conjugate does not induce hyporesponsiveness
to subsequent 23-valent polysaccharide vaccine or to a second dose of conjugate
vaccine. Therefore, conjugate could be
used to extend age range of protection against pneumococcal disease, for
example down to 50 years of age and to provide long term protection by repeat
dosing if needed.
So
those statements are based on data that we have collected from a pilot study
done with Prevnar, the 7-valent vaccine
in Germany in elderly patients 70 years of age or older not previously
immunized with a pneumococcal vaccine.
In
year one patients were randomized to receive a 7-valent conjugate versus the
23-valent polysaccharide vaccine.
Antibody measurements were done before and after immunization. A year later the pneumococcal conjugate group was rerandomized to receive either
a second dose of pneumococcal conjugate or the 23-valent polysaccharide. The polysaccharide group was not
reramdonized; all of them received pneumococcal conjugate vaccine.
This
shows you the immunogenicity by ELISA, geometric mean titers. In blue to the conjugate, in red to the
polysaccharide. And the mean antibody
concentration were significantly higher, about two fold to three fold after
conjugate for all but one of the types, which is type 19F where the difference
was not significant.
Now
we've talked a lot about functional antibody concentrations and so shown here
are the opsonic titers to the same seven types with Prevnar and 23-valent
vaccine. Again, you see similarly that the opsonic antibody activity is higher,
two to three fold, and because the higher variation of the assay that reaches
significance for four, not six of the seven types.
So
another question we were interested in asking is does prior polysaccharide
effect the response to pneumococcal conjugate vaccine? And to answer that question we looked at the
lower group circled where pneumococcal conjugate was given after polysaccharide,
one year after polysaccharide. And as a
reference we looked at pneumococcal conjugate given initially without prior
immunization.
And
shown here in red is what happens to 7-valent responses after polysaccharide,
one year after polysaccharide. And you
can see that they are significantly lower for most types than when pneumococcal
conjugate is given to a naive individual.
This period of time is only one year.
So immunogenesis cannot account for this. This is immunoresponsiveness
which the conjugate vaccine was a probe to uncover, if you will, in this study
design.
So
Prevnar -- 7-valent vaccine blunts the response to subsequent Prevnar. So then the question is does Prevnar blunt
the response to a second dose of Prevnar, and the answer is no it does
not. And the green is Prevnar given as
a booster dose, if you will, one year after the first dose versus in blue
7-valent given up front. And the
responses are essentially the same.
Another
question is does giving pneumococcal conjugate effect the response to a
subsequent dose of polysaccharide. And
for this comparison we looked at polysaccharide given after pneumococcal
conjugate in the circled group. And
compared them to those who got polysaccharide up front. And what you see here in yellow are
responses to polysaccharide after conjugate, and as you can see, they are
generally somewhat higher than with 20 polysaccharide initially, but not
significantly so with the size of this study.
But certainly we don't see hyporesponsiveness induced by Prevnar for
subsequent polysaccharide.
Now
a question we wondered about is since there was only a one year interval
between these immunizations whether this hyporesponsiveness would persist over
a longer period of time. And what I'm showing you here are data from Lisa
Jackson's study as yet unpublished but with her permission in which the
interval between polysaccharide and conjugate was 5 years or more. And in her
study individuals received either conjugate in green or polysaccharide in red. And focusing on the conjugate responses you
can see that they're actually remarkably similar to the responses we saw in a
separate study, different country but similarly aged patients suggesting that
probably longer intervals won't mitigate the hyporesponsiveness that we see
after 23-valent polysaccharide vaccine.
And
this just to answer a question, actually, that was raised earlier. With repeated doses of polysaccharide
vaccine, this shows you the responses. The first two points here are the
response to the first dose of polysaccharide.
Then the next point is a year out. The fourth point is three to seven
years out. And then a second dose of polysaccharide is given and you see the
responses of that. And it's clear that for four of the six types that were
examined there is a significant reduction in the ability to respond with the
second dose of a polysaccharide which has been termed
"hyporesponsiveness."
So
the data I've shown you on immunogenicity I think support the following:
First
of all, that Prevnar conjugate can be used repeatedly without inducing
hyporesponsiveness in the elderly.
Second
of all, that 23-valent polysaccharide can be given after pneumococcal conjugate
vaccine without hyporesponsiveness.
And
if both vaccines are used to maximize coverage, conjugate should be used first.
The
third question is what is the potential public health impact of pneumococcal
conjugate vaccine for adults? Now, you
need to make a series of assumptions, and in your briefing package these
assumptions are outlined in a lot more detail than I will here. But to
summarize the assumptions we made were that serotype coverage based on the 2003
incidence of disease in the U.S., so it takes into account to a large extent
the herd immunity effect of Prevnar, is 75 percent currently for 23-valent
polysaccharide vaccine and 56 percent for the proposed 13-valent conjugate
vaccine.
Invasive
pneumococcal disease rates are, again in the briefing package, but they do
reflect the herd immunity effect of Prevnar. But what was done was to back out,
if you will, the effect of the use of 23-valent polysaccharide using
assumptions that were in a paper published by Fry, et.al. So they actually adjust upwards slightly
assuming 23-valent is not being used.
We
assumed then that the efficacy for a pneumococcal polysaccharide vaccine would
be 88 percent for five years. That's
based on the Shapiro study. And
thereafter declining to essentially zero percent by about 15 years.
In
contrast we assumed that for 13-valent vaccine efficacy would be the same for
polysaccharide but could be maintained at the similar level throughout the risk
period.
We
assumed neither vaccine would be efficacious for the immunocompromised
patients. And the vaccine uptake, the
assumption was the current level of update that we have achieved with
23-valent, which is 60 percent in over 65 years old, 43 percent in high risk
groups under 65 and zero percent in healthy under 65. In contrast 13-valent conjugate uptake would be 60 percent from
50 years onwards.
Using
those assumptions one can then estimate of numbers of cases prevented and in
parenthesis deaths prevented by these vaccines. The 23-valent vaccine shows a low level of prevention from using
it in high risk individual under 65 and then a peak of protection assuming
everyone gets immunized. And then
weaning prevention over time. And so
the net effect of all of that is calculated to be under 3,000 cases prevented
and a little under 500 deaths prevented overall per year.
If
one were to use a 13-valent alone and assumed with potentially repeat
immunization one maintains protection at 88 percent throughout the high risk
period. One would prevent, despite the somewhat lower coverage of 13-valent,
almost twice as much, 86 percent more cases of disease and deaths.
Now
it's possible, as we mentioned, to give the 13-valent first followed by
polysaccharide and get the advantage of the additional serotype coverage that
way. And the additional cases prevented by doing that are 566 with about 93
deaths. And the total number of cases prevented, as indicated, is over 6,000
and almost a 1,000 deaths.
Now
these estimates are really quite conservative in terms of what the public
health impact would because we don't assume any IPD efficacy despite the fact,
as I've shown you, that we have higher ELISA and OPA antibody responses. We
also don't assume any protection for the immunocompromised groups although
there are data. In HIV positive
patients, for example, the responses to conjugate are significantly better than
they are to the polysaccharide as well as in other high risk groups such as
renal dialysis patients, individuals who have been shown to be hyporesponsive
to polysaccharide subsequently immunized with conjugate that respond and so
forth.
It
also assumes no efficacy for pneumonia even, as I'll show you in a moment, the
OPA antibody after pneumococcal conjugate in the elderly is actually similar to
OPA antibodies after three doses in infants.
I
want to emphasize here that we are not making the case nor or we requesting
that there been an indication for pneumonia. That may be a benefit of a
vaccine, but we don't believe that we can demonstrate that prior to
licensure. Rather, we're going to make
the case that we bridge to polysaccharide, which we know to be effective in the
elderly population and in the adults.
Okay.
Now
the fourth question is are serologic studies adequate to demonstrate efficacy
of adult pneumococcal conjugate vaccine?
Historically there have been two approaches used for licensing polysaccharide
based vaccines, whether polysaccharides or conjugates. First of all, when there
is no vaccine to prevent the disease in the particular age group, an efficacy
trial is required if feasible. And
examples of this from the past are the 14-valent polysaccharide vaccine, the
Group A and C meningococcal vaccine, the Hib polysaccharide vaccine in
toddlers, which we licensed based on the Finnish efficacy trial, the Hib
conjugate vaccine in infant based on Navaho and Kaiser trials and the
pneumococcal conjugate vaccine in infants based on Kaiser. However, when there is already a licensed
vaccine to prevent disease in particular age group, immunogenicity comparison
has been acceptable to extend the coverage to other serotypes or to improve the
level of immunogenicity by switching to conjugate from polysaccharides
And
examples of that are the 23-valent pneumococcal polysaccharide after 14
extending serotype coverage, the 4-valent meningococcal pneumococcal after
2-valent, again to extend serotype coverage, the Hib conjugate vaccine after
Hib polysaccharide vaccine in toddlers to achieve better immunogenicity. There was no efficacy trial done for that in
toddlers. And very recently, as was mentioned earlier, the 4-valent
meningococcal conjugate vaccine Menactra after 4-valent polysaccharide vaccine
based purely on serology, no efficacy trials.
So
the proposal for licensing adult conjugate then is based on the regulatory
precedents that the efficacy of a pneumococcal conjugate for adults can be
proven by showing a serologic non-inferiority to the shared serotypes in the
licensed 23-valent polysaccharide vaccine based on OPA assays.
Secondly,
that there be lack of hyporesponsiveness to second dose of conjugate vaccine
which will enable repeat doses if needed to maintain protection.
And
thirdly, that there be a lack of hyporesponsiveness to 23-valent polysaccharide
vaccine given subsequently, which would enable extending serotypes coverage in
high risk groups if so desired by advisory committees.
Now,
the scientific basis for serologic studies showing efficacy of this vaccine is
as follows:
First
of all we know that the efficacy of the 23-valent vaccine is established and we
know that the only antigen in that vaccine that could provide protection is the
capsular polysaccharide. So the
polysaccharide is a protective antigen. There's no question about that.
Second
of all we know that antibody is the protective mechanism against invasive
disease. There's no question about that
either. Passive immunoglobulin therapy protects against pneumococcal invasive
disease.
Thirdly
we know that opsonophagocytosis is the protective mechanism. At the risk of sound dogmatic, there is no
alternative mechanism whereby antibody can protect that's known.
Fourth,
induction of opsonophagocytic activity is believed to correlate with clinical
efficacy and is proposed as a primary basis for comparing adult vaccines. Now, I'll show you a little bit more
information from which we could infer that that's a reasonable hypothesis. I think absolute proof, it would be hard to
come by.
And
five, antibody binding assays such as ELISAs can be used as surrogates when
they correlate highly with OPAs, as is the case in infants where the
correlations are very high. Our
experience, like that of others who have spoken earlier, that is in the elderly
that correlation isn't very high, it's rather low. And therefore OPA
measurements are probably more appropriate as a direct measure.
Now
just to review what others have mentioned before is that there is very
substantial evidence, convincing evidence that the polysaccharide vaccine is
efficacious for invasive disease. There is much less convincing evidence, as
others have also commented, that it's efficacious for pneumonia in the elderly,
and therefore when we bridge to polysaccharide we can only expect to bridge to
it for an invasive disease indication.
Now,
why is OPA the appropriate laboratory measurement to use in adults? Well, we know that OPA in infants is very
high and efficacy of this conjugate vaccine in infants was also very high. And
so the high OPAs appeared to correlate with high efficacy.
Of
particular interest, though, is one of the types, type 109F, has lower OPA in
infants than the other six types. And
although the efficacy of Prevnar for 19F is quite high, it is lower for otitis
media and for inhibition of 19F colonization.
And it seems to relate to the low OPA.
And let me show you the data on which those statements are based.
Shown
here at the ELISA titers, geometric means after three doses of Prevnar at seven
months of age in infants on the left column and then the OPA titers on the
right.
And
you can 19F stands out as having a low OPA titer relative to all the other
types. And so the question is does that correlate with anything clinically. And
the answer, it does seem to.
Now
for invasive pneumococcal disease it's not very dramatic, although it's true
that both in the Kaiser study and in the ABC case controlled surveillance that
was done more recently, the 19F point estimate of efficacy is the lowest of all
the seven types, 85 percent and 81 percent respectively.
Otitis
media where the demand on having antibody is probably greater shows this lower
protective activity better. And here
19F has only 25 percent efficacy. Much lower than the other six types. And for colonization as well, and this is
just data in Israel, 21 percent. In
fact, it's quite striking looking at the data how well colonization
inhabitation correlates with otitis media efficacy.
OPA
also explains what has been to many of us a conundrum, which is why do the
elderly who have reasonably good binding to antibody activity have such a high
risk of disease. Specifically elderly
adults have similar ELISA antibody levels even prior to immunizations as infant
do after Prevnar. And yet they are at
very high risk of invasive pneumococcal disease. The explanation, as you already heard also from Jan Poolman, is
that pneumococcal antibodies in the elderly have lower opsonic function
relative to infant antibody. And I will
show you some more data on that.
So
first of all on the point of what the elderly ELISA antibody concentrations are
even prior to immunization, shown on the right here are elderly unimmunization
individuals, geometric concentrations, all around a microgram. And then in infants after three doses. They
are higher, but not a lot higher. And
if one used the infant derived population based estimate of protection of .35,
the WHO Committee has suggested, most of the elderly should be protected and
apparently they are not.
If
you now look at the OPA titers in red you see the dramatic difference in OPAs
between the elderly and the infants. And we propose that this difference is
what predicts the fact that the elderly without immunization are at risk.
So
the quality of the antibody in the elderly is much less than in infants. However, after a single dose of Prevnar in
the elderly there is an increase in OPA antibody titers to levels similar to
that in infants after three doses. And that increase involves both quality
improvement as well as absolute concentration improvement.
Shown
in black is the ELISA antibody concentration in the elderly after
immunization. And what you can see is that they're actually higher than
in infants by substantial amounts in many cases. And the OPA antibody now is
similar to infants, albeit the quality, the functional quality of OPA activity
per microgram of antibody in the elderly is lower. But the net OPA is similar.
So,
again, the proposed licensing criteria for adult pneumococcal conjugate then
are to demonstrate non-inferiority of the immune response of the shared
serotypes in the 13-valent conjugate and 23-valent polysaccharide with the
primary comparison being based on OPA.
To
demonstrate no hyporesponsiveness to a second dose of 13-valent, and this will
support repeat dosing of the 13-valent for long term protection if that's
needed.
And
to demonstrate no hyporesponsiveness to subsequent dose of 12-valent. And this
would support a recommendation to use 23-valent polysaccharide to extend
serotype coverage in high risk groups, if desired.
So
the final question is whether an efficacy trial is feasible for invasive
pneumococcal disease or for community acquired pneumonia. And I think, as speakers before me have
mentioned, there are a number of constraints on performing pneumococcal
conjugate vaccine efficacy trials in adults for CAP or IPD. A placebo controlled trial is necessary if
we are to assess in any true sense the efficacy of 13-valent vaccine. Placebo is not possible in high risk adults
who are currently recommended to receive the 23-valent vaccine. And that means over 65 and those under 65
with the high risk conditions for which the polysaccharide is indicated.
Therefore,
only healthy healthy less than 65 year olds can be studied. In this age group
72 percent of all invasive disease occurs in the high risk portion, which would
have polysaccharide. So we're left with IPD rates in the healthy less than 65
year olds that will be much lower than those for the entire age group. And those have been generally used for the
calculations we've heard so far. They
will be lower in the healthy group.
So
as a result studies of IPD or CAP in those groups would require absolutely
enormous sample sizes in excess of 100,000.limb for adequate power. A variety of alternative designs have been
discussed such as using a combination of 13-valent polysaccharide versus
23-valent alone, and then being able to do it in high risk groups. But if you use IPD as the outcome with a
somewhat efficacious 23-valent vaccine, those study sizes would be even larger
than the ones we're calculated.
So
post-marketing effectiveness studies are really the only feasible way, in our
opinion, to assess the impact of 13-valent vaccine on IPD and possibly on CAP.
And we've seen very elegant work from the ABC system described this morning of
how effective our ability is to look at IPD rates and incidents over time.
So
but just to go through the exercise, and I think Doug Pratt did so this morning
as well, with a few I think more realistic assumptions about rates, what would
the sample size be for IPD in 50 to 64 year old healthy adults? And our assumption of an incidence rate of
vaccine type disease, vaccine type disease is 25 per 100,000 or as a high rate,
and that's be a very high rate, 15 per 100,000 as an intermediate rate and 7.5.
per 100,000 as a low rate.
And
we should note that the CDC estimates Prevnar in healthy 50 to 64 year olds are
9.9 per 100,000 rate. So I think now
with herd immune effects and only vaccine coverage of 56 percent, the 7.5 is
probably the realistic rate we could expect in this study population for
IPD. We assume 56 percent IPD coverage
by 13-valent. We try vaccine
efficacies, true efficacies of 70, 80 and 90 percent; 90 percent power. Lower 95 percent confidence intervals
greater than 30 percent and a realistic trial length of a total of three years;
one year to enroll, two years to follow-up, a mean follow-up time of 22 years.
So
with those assumptions this shows you the numbers of patients per limb that
would be required to achieve an adequately powered trial. Now we can dismiss
the 25 per 100,000 estimate as being unrealistically high for a healthy 50 to
64 year olds. So look at the 15 and the 72, and I think 90 percent efficacy is
unrealistically high as an expected benchmark in the elderly as well.
So
the red figures are the numbers that we ended up for possible trial sizes. And we believe that in healthy 50 to 64 year
olds they will not be possible to do trials of that size.
Without
going into figures, but there are a variety of major issues with CAP
outcomes. Again, we can ethically only
say healthy less than 65 year olds here, and probably much of the CAP incidence
in the 50 to 65 year old group that is talked about is in high risk
individuals. So the CAP risk will be low and sample sizes will be extremely
large.
We
don't really know the proportion of CAP that is due to pneumococcus, and so
that makes estimating sample sizes uncertain and increases the risk.
The
etiologic diagnosis of pneumonia would enable a smaller sample size. There's no question about that. But unfortunately, there is no validated
method available today to do that. And if your method picks up cases that are
false/positives in your control group, the sample sizes would be driven even
higher. And for us, the lack of a validated outcome is a show stopped for
vaccine type CAP efficacy trials.
And
finally, as I mentioned before, I think our ability to enroll very large
numbers of healthy low risk individuals into such trials I think would be
limited.
So
my conclusions are that 13-valent pneumococcal conjugate vaccine has the
potential of a significant public health impact because it can extend the
duration of protection throughout the high risk period.
The
23-valent polysaccharide vaccine may be given after the 13-valent pneumococcal
conjugate vaccine to expand serotype protection in the high risk groups.
Efficacy
of a conjugate vaccine in adults can be proven by showing non-inferiority of
the immune response to the licensed polysaccharide vaccine for the serotypes
that are in the conjugate. Placebo
controlled efficacy trials in the adult population are not feasible due to
ethical considerations and size.
And
effectiveness against IPD can be confirmed in post-marketing studies.
Thank
you.
CHAIR
OVERTURF: Dr. Markovitz?
MEMBER
MARKOVITZ: Yes. Because you guys make Prevnar, I hope you're
the right person to ask this question.
A number of us were talking about this over lunch. And what I haven't
seen yet and it didn't come up in your data, obviously with adults we really
don't know, but even with the kids in the initial trials you did that showed
that Prevnar was successful, were you able to actually look at kids who did get
pneumococcal disease and show that they had lower opsonophagocytic
responses? Are there any data actually
to really address whether there's a correlation here? Because like what you showed here, pointing to that one serotype
where you had lower levels and was somewhat less efficacious, it appeared that
the levels were considerably lower but yet the efficacy was only marginally
less. So do you actually have data from
that original trial that could help us to at least understand whether this test
is useful in some setting in a more definitive way?
DR.
SIBER: Are you asking about data prior
to disease?
MEMBER
MARKOVITZ: Yes.
DR.
SIBER: We do not have such data with
pneumococcal disease. The problem with
that is that you have to bleed every child in a very large efficacy trial, and
that has not been done.
There
are some examples where such sera are available, but they're anecdotal. One of the best ones is from the Hib
efficacy trial conducted on a Navaho reservation where they did bleed every
child, I believe, and they had a serum on a child who subsequently became ill
with Hib disease. And what you
typically find in this setting, and there's some examples, I actually reviewed
this a few years ago, is that the antibody levels of those who end up getting
sick are now lower. They fall in the
same range of those who are protected.
And
the notion that you can simplistically look at somebody's antibody level
individually at a particular time and expect to predict individual based
protection is false. Can't do that. You can do population based protection
estimates. We cannot reliability on an individual basis predict protection.
MEMBER
MARKOVITZ: But what about looking at
the kids who got -- but I guess perhaps I didn't ask that question properly.
What I really want to know, and apparently there are no data but correct me if
I'm wrong, has there been an analysis of the levels of those antibodies overall
in kids who did get sick versus those who didn't get sick? I assume not because
you didn't bleed everybody.
DR.
SIBER: Right.
MEMBER
MARKOVITZ: So the answer really is
there are no data to directly address this question?
DR.
SIBER: Not prior to illness.
MEMBER
MARKOVITZ: And did you have data after
the illness, though?
DR.
SIBER: No. I don't think so. I'm not
aware. Maybe there are such data. I'm not aware that people have collected
systematically data of breakthrough cases to look at the antibody
concentrations with the pneumococcal vaccine.
CHAIR
OVERTURF: At the microphone. Just identify yourself.
DR.
POOLMAN: Jan Poolman from
GlaxoSmithKline.
And
we actually did that in the situation of a no otitus efficacy study where the
number of children involved are lower, so you can have your prebleeds. We still have to publish. But your children that came down with otitus
media later on, for the few serotypes where we had sufficient cases in each
case for each serotypes there were about three or four serotypes, has
substantially lower opsonophagocytic antibody levels.
DR.
STEINER: Sandy Steiner from CDC. We
also have a comment on that.
The
Navaho trial that was done with Kate O'Brien there was one child that we
happened to have serum also before, throughout the bleeds. One of them was
vaccine failure. I'm trying to remember the serotype, but I think it was
19F. And -- or 14 actually -- was 14
serotype. And we'd like at the titers, the opsonophagocytic titers and they
were reduced by the single serotype killing assay. When other assays were looked at actually, it was not
reduced. But for the killing assay it
was significantly reduced of opsonophagocytic titer.
And
it also had lower avidity. It happened
to be the child that had the lowest avidity of all the controls that were run
along with this child.
This
study still has not been published and we're working on the publication with
Kate O'Brien, so it's very confidential.
MEMBER
MARKOVITZ: I'm sorry. Are you
differentiating between phagocytosis and --
DR.
STEINER: But we need to know these.
MEMBER
MARKOVITZ: Thank you. We'll keep it
quiet then.
DR.
STEINER: Yes.
MEMBER
MARKOVITZ: May I ask, did I understand
right, are you differentiating though between phagocytosis and killing are you
using those synonymously.
DR.
STEINER: No. Measuring of phagocytosis by the killing assay. Measuring.
Yes.
CHAIR
OVERTURF: Dr. Steinhoff, you had a question?
DR.
STEINHOFF: Well I'm going to change
the subject. I don't know if there's
another one about OPA. As long as you
call on me later.
CHAIR
OVERTURF: Dr. Hetherington then?
DR.
HETHERINGTON: This may be short.
Dr.
Siber, if we agree that older adults have a deficiency in OPA, do you have any
sense as to where that deficiency lies?
For instance, is it the sub blast distribution of the antibody response
knowing IGG4, for instance, is opsonic?
DR.
SIBER: I would be really speculating
about how it happens. I think there's some hypothesis you can generate based on
what we know. If you believe that
polysaccharides induce hyporesponsive, we showed you some data that they may.
Over time we see the pneumococcal polysaccharides many times. If each time
polysaccharides drive your B-cells to make antibody without replenishing memory
cells, you can imagine over time that the memory cells of your best clones
become less and less and you start recruiting not so good clones, and those may
have less opsonic function. That's a
hypothesis.
DR.
POOLMAN: Once more, sorry. Jan Poolman, GlaxoSmithKline.
And
there are two very recent publications in effect immunity, from Julie
Westeringsteam. She shows that in the
elderly the variable regions of both the heavy chains and the light chains are
substantially different as compared to the adults, which must translate into
functionality, like it clearly does.
DR.
SIBER: It's very consistent with the
hypothesis I just mentioned.
CHAIR
OVERTURF: Dr. Steinhoff?
DR.
STEINHOFF: It's interesting to hear
this because I was going to raise the issue, George, that you very early on
showed the age distribution of disease which has a U shaped curve increasing in
adulthood. And I was not aware of this
data that the nature of the antibody changes in the elderly. Because the level doesn't. The antibody titers stay pretty much the
same for age 20 to age 50 or 60. So the question is is it the antibody that
changes, and perhaps it does, but I also wondered if the cellular function
doesn't change? And that would account
for titers that are about the same but function that is much less. Because the
other limb of the OPA is the white cell function. And maybe they both change.
DR.
SIBER: Well, I think you're right that
the quality of the antibody very clearly changes. And I think our best measure of that is the opsonic functions
falling.
You
know, I can't speak to the white cell function in the elderly. I don't think we
have data one way or the other on that to my knowledge.
CHAIR
OVERTURF: What about affinity
specifically, which is another measure of antibody function? Has that been
looked at?
DR.
SIBER: Dr. Steiner, you may have data
on affinity in the elderly. I don't think we do.
DR.
STEINER: Yes. We have the publication
from 1999 and that was on the elderly where there was very low -- measurements.
It was affinity, it was a -- measurement. And it was very low if you measure it
in molarity for -- compared to the young adults. It was in the range of less
than .1 more. And for the young adults
it was in the range of 1.1 to 1.3. So
it's like a ten fold difference. And it
also correlated with function. Those that had the low of the antibodies did not
have function and those with the higher had high function.
That's
the same study that was done in adults by Lucas, Alex Lucas. And even though they were not elderly, it
confirmed the studies that we had done on the same year.
One
more question. There was a question regarding the B-cells. And in 2005 there was a publication that
just got published in infection and Immunity and Aging is the
journal. And with Dr. Westerings
group. And we collaborated.
We
saw that also the numbers of these cells that are present in the elderly are
lower in the very elderly in comparison to the normal young adults. So the
numbers of cells, not only the clones maybe lower that are present, that's
something that we should also consider looking into.
CHAIR
OVERTURF: I think Dr. LaRussa was first
here.
MEMBER
LaRUSSA: Just to comment and then a
question. In a number of the examples
that you cited where we were able to approve a vaccine based on inferiority to
something that was already there, I just want to remind people that in two of
the examples we were essentially adding on to what was already there covering
more serotypes. So you could argue that even if the additional serotypes didn't
work, you weren't subtracting anything.
In
the case of hemophilus we knew what the correlates of protection were. So that really doesn't count. And I guess
the one example where you could say we really did add a vaccine on the basis of
non-inferiority was the meninga
example. So that's just a
comment.
I
want to go back to one of the scenarios that you dismissed for efficacy. And
what I would argue is that in the age group over 65 you really could revisit
the scenario of giving conjugate first and polysaccharide second and studying
efficacy against community acquire pneumonia.
Because we don't really believe that the polysaccharide works that well
against pneumonia. And although it would be a large trial, it really would answer
the question of efficacy in the age group where we really need that question
answered.
So
I wouldn't dismiss that. I would think about that more seriously.
CHAIR
OVERTURF: Dr. Karron?
MEMBER
KARRON: Partly as a follow-up comment
to that, I think I had a question
about, George, you're saying that a placebo controlled trial would be necessary
to test efficacy, particularly thinking specifically about CAP since we don't
really think in people over 65 there's appreciable efficacy of the
polysaccharide vaccine. So whether you
have the kind of scenario that Phil was suggesting of sequential immunization
or whether you had a head-to-head comparison, would that be possible?
And
the second question I had for you is what about the issue of doing an
effectiveness study for CAP? I mean,
would that be feasible? I understand
that definitive diagnoses is difficult, but is that feasible?
DR.
SIBER: Well, I think the numbers would
be enormous, but I think beyond the numbers, even in the high risk population
over 65 the difficulties we've encountered with pneumonia outcome are best
illustrated maybe by the debates we've had about even the pneumonia efficacy of
this vaccine in infants. And I would
remind the group that we have not been able to agree amongst the regulatory
agencies, investigators or WHO on a definition that we all agree is pneumonia.
And that's in infants, where it's relatively straightforward, in my opinion,
compared to older people with their background of x-ray issues.
And
as we talked about earlier, the outcomes with regard to microbiological
documentation are problematic. We
simply don't have a validated way to make a pneumococcal diagnoses.
So
we are left with a situation we're very uncertain about how we could agree on
an outcome for a pneumonia study in any kind of study. And on top of that we have the issue, I
mentioned that the huge sample size required even with the current rates of
CAP, if you accept those as real and those come, I believe, primarily from
diagnoses put into charts by doctors.
So
I think you're left with a tremendous amount of uncertainty in designing such a
trial, and a tremendous sample size to do it.
Also,
all of you are reasoning that pneumococcal polysaccharide does nothing to CAP.
I think there's been a lot of debate on that issue. It may do something, it may not do something. The power of most studies have not been
adequate, really, to address the issue.
So if we powered a study at the size we're talking about, hundreds of
thousands of individuals, there'll be this uncertainty about what the
pneumococcal polysaccharide control did.
And so you're left with some uncertainty there for what conjugate
efficacy would be.
CHAIR
OVERTURF: Dr. Jackson?
DR.
JACKSON: Yes. I was shifting gears a
little bit. I was looking at your model demonstrating the estimated public
health benefit of a conjugate program versus current status of using the
polysaccharide. And most of the
relative benefit of the conjugate vaccine program occurs at prevention of cases
in pretty the very elderly, 75 and 80 or 80 and over. And I think although
certainly tolerance has been a concern, but part of the reason that we don't
have routine revaccine may also be because of concern that there's a lack of
primary immune response or a lack of effective immune response in persons in
their late 70s, 80s and older to the polysaccharide vaccine. So it does raise one question, which is
what's the mean of non-inferiority in an age group in which perhaps we're not
so sure what we've currently got is terribly effective.
And
the second is what would you propose to do to ensure or to try to try to
estimate of the conjugate vaccine in this older end of the age spectrum where
most of the disease is occurring?
DR.
SIBER: Well, I think non-inferiority is
what we would formally propose, and that's a really a regulatory convention to
look for non-inferiority. That's a requirement. And my opinion is the minimum
requirement. And as I've shown you, we are actually seeing a significantly
higher responses with conjugate versus polysaccharide. And we assess the
13-valent properly in this setting we would hope to see the same similar higher
response.
In
terms of showing the impact, I am very confident that the ABC system, which
really looks at disease in all age groups, will provide excellent data but it
requires the vaccine to be introduced and used. But we will find out what the impact is over time through
ABC. And that will be the best data
that we can hope to expect.
CHAIR
OVERTURF: Last question. Dr. Farley?
MEMBER
FARLEY: I think many of us are sort of
grasping on to trying to get some clinical outcome as part of this measurement.
And I'm curious to hear your comments on what you think the role of
colonization studies might be assessing this in adults, realizing that the
carriage rates are going to be lower in adults? But do you think that would have any benefit or play a role in
assessing pre-release of this vaccine?
DR.
SIBER: No. I think it would be very
interesting to try to show an effect on colonization in adults. As you point
out, the big problem that in the absence of children in the household, the
studies of colonization are from one to five to six percent. Then when you
consider what proportion of those will be vaccine serotypes, that also will be
an extremely difficult undertaking to do that.
It's something we would like to look into further.
We've
also recognized the position that I think Doug Pratt enunciated this morning is
that although colonization is interesting, patients are not clinically ill with
it and it would probably not be a basis a licensure now. That's our understanding. And so the value of the colonization studies
from that vantage may be limited.
CHAIR
OVERTURF: Thank you, Dr. Siber.
We
need to move on to our last speaker before we proceed with questions. So I'll ask Dr. Fries.
DR.
FRIES: Okay. I will try to make this a
fairly abbreviated talk. Obviously, I'm not going to replow a lot of the ground
that has been covered so ably by Drs. Poolman and Siber.
I'm
a rather unique representative here in that I'm representing a protein,
hopefully, group common protein vaccine as opposed to a vaccine based on
pneumococcal polysaccharides. And as
such, the considerations and the regulatory avenues that are open to me are
profoundly different.
Let's
just quickly go through some of the first slides, then I think the meat of what
I have to say is in the second half of this. Because much has already been
said.
In
terms of the U.S. burden of pneumococcal disease in the elderly, which is the
group we're focusing on, as has been said by so many, it breaks down into two
categories, really. Invasive disease
which is a mixture of bacteremia without a focus, pneumonia with bacteremia and
relatively uncommonly in the elderly, meningitis, but it's certainly there with the cited levels of incidence of
disease and mortality. It does have a
disproportionate impact among blacks and, obviously, occurs with an increased
rate in the risk groups everyone has identified.
The
other target of opportunity and of interest is, obviously, community acquire
pneumonia or CAP. Somewhere between 350
and 620,000 hospitalizations per year. We do not know what proportion of that
is due to pneumococci. You'll see
estimates everywhere from 20 to 60 percent, I would say. One would be very brave to actually assume
it's above 30 percent, and so I won't.
You've
seen this before. The indirect impact
of the conjugate vaccine administration to children and the elderly with the
declining rates of IPD in the elderly since the introduction of the conjugate
vaccine. In children we know there is an increasing rate of non-vaccine
serotypes, as is shown in the right hand panel. And in Lexau's most recently published data, which has been
referred to earlier, what we can see is that the upper portion of those bars in
2001 and 2002/03 which represents the non-vaccine serotypes and the serotypes
which are represented solely by the polysaccharide vaccine are sneaking up in
absolute rate in the elderly population even as the absolute numbers are declining
in response to the conjugate. In fact,
over this period of time that increased absolute rate is actually some 11.6
percent. This is a very short term
experiment, an observation, but obviously the behavior of those upper two
pieces of the pie there deserves continued observations and is one of the
things that interests us in approaching base vaccine.
Evidence
regarding pneumococcal vaccines in the elderly has been outlined fairly
carefully. I will not spend a great deal of time on it. In terms of invasive disease, there's no
compelling evidence from randomized trials in the elderly. South African gold
miners, yes. But not the elderly. Meta-analyses are heterogenous and they're
still underpowered, but obviously the vast burden of observational cohort in
case control studies monotonously show somewhere between 45 and 65 percent
efficacy. And I don't think anyone's
going to question that.
For
community acquire pneumonia, however, there's no evidence in controlled
studies, again. Observational studies
are heterogeneous often, although not always, quite underpowered. Meta-analyses aren't particularly helpful
either. So there's a suggestion of an impact but the data are variable and they
don't point as strongly in any direction.
In
terms of cost effectiveness the 23-valent vaccine is generally believed to be
acceptably cost effective in the elderly.
There have been a variety of analyses featuring multiple different
assumptions, but all of them suggest that it's cost effective. Essentially based
on IPD alone.
Now,
as I said earlier, ID Biomedical's approach is fundamentally different. Our
candidates are chimeric protein, which represents immunodominant and
surface-exposed domains and, (2) conserve pneumococcal proteins in a fusion
protein. It's current configuration is
an aluminum adjuvanted injectable. We do believe it's capable of development in
both aqueous formulation, which we're looking at particularly for the elderly
where it's actually proved quite promising.
And I will potential for mucosal formulations. We haven't gone there but
it's something that the protein nature of the vaccine opens up as a
possibility.
Now,
why go to a protein after all, and particularly a group common protein? And in this table I think we look at some of
the features.
In
terms of serotype coverage whether you have a polysaccharide vaccine or a
conjugate, you always have to some extent the limited array of serotypes that's
possible to cover. And you can be
victimized a little bit by geographic diversity in terms of how good your
coverage is in any particular area.
For
a group common protein based vaccine you can potentially cover all
pneumococci. And our studies to date
suggest that our antigens are expressed on 99 plus percent of over 400 strains
that we've tested so far, and we're still going.
Serotype
substitution has been discussed extensively in terms of what's already happened
in children and the suggestions that are occurring in adults. We don't really know yet its importance in
adults, but with a group common protein based vaccine serotype substitution is
not an issue.
On
the other hand to be fair the possibility of escaped mutants in a protein is an
issue. That's not the case with a
polysaccharide vaccine. So that's a little black mark that has to be followed
carefully with our product. One of the things that we hope helps avoid
that is we include sequences from two separate proteins in the product.
In
terms of the complexity of manufacture, ours is relatively low. It's a single
high yield recombinant product. And
certainly the complexity of manufacturing releases has to be higher for
conjugate -- for polysaccharides of any sort, but especially for conjugates.
T
cell help with our product is intrinsic, it's a protein. For polysaccharides you require conjugation.
And
as a correlate of that our early data, at least, suggests that this product
boosts very effectively at short intervals and at longer intervals in the
elderly and is quite safe doing it, whereas boosting, as you've heard, with the
23-valent polysaccharide is mediocre, to put it generously, with some safety
concerns. And it's certainly better for conjugates.
Last,
but not least, we feel we have a strong potential for eliciting a mucosal
immune response.
Without
going into great length of data, we have carried out a number of clinical
trials. And as part of those clinical
trials we've been able to show passive protection in animal animals with doses
of antibody from immunized subjects that would provide about 5 microgram per
mil of antibody to the conjugate antigens in the animals. This happens to be data from a lethal
pneumonia model where we've been able to show about a 10,000 fold reduction of
bacterial counts in the lungs of immunized animals. You can see similar results
with a sepsis model. And this can be
done both as active immunization and by passive transfer of immunized human
serum.
And
without going into details, the basic mechanism of protection appear very much
the same as those induced by the current vaccines. You have complement, dependent and phagocyte dependent,
opsonophagocytosis. You can absorb out
the specific antibody and it goes away.
So it's antibody complement in phagocytes, much as the polysaccharide
vaccines.
Now
having gone through that there are quite a string of challenges and different
challenges in the development of a pneumococcal group common protein
vaccine. There's, obviously, a vastly
smaller amount of date, although we're actively gathering it regarding the
prevalence of protein antibodies in the normal healthy and ill human
populations and their relationship to underlying disease rates.
Current
assays of functional antibodies which you've heard discussed at great length
here, are opsonized for polysaccharide antibodies. And when we try to use these same assays with our product, we get
a single but it's profoundly confounded by the presence of polysaccharide
antibodies. And sorting it out and opsonizing the assays to detect the
induction of opsonic activity specific for these proteins you have to ring
changes on the assay, which is already the product of decades worth of
optimization and validation.
There's
certainly no consensus regarding the protective level of any pneumococcal
protein antibody. And to the extent
that there's argument with polysaccharides, there's no information with regard
to these proteins and antibodies to them.
And
lastly, and to us the major concern is that we think that clinical trials for a
licensure of this product in the elderly or, for that matter, in the young will
undoubtedly require clinical efficacy. But for some of the reasons you've heard
in Dr. Siber's presentation, we're going to have to do some new thinking about
endpoints that would lead to feasible clinical trial designs. Clinical trials targeting invasive
pneumococcal disease will be huge. I was glad to see that Dr. Siber's numbers
validated my estimate that we'd be somewhere between 300 and 600,000 subject
years of observation to show efficacy against invasive pneumococcal disease in
the elderly.
If
you do trials looking at all cause CAP, they're actually better than the IPD
trials in terms of size, but they're still dauntingly large because of limited
of efficacy attainable. I would
question whether it's really rational to posit 90 percent efficacy against an
illness in a heterogeneous population
of people with comorbid conditions, and elderly. And that being the case, you're looking at reductions of a
fraction, 15/20 percent efficacy at most in CAP trials. So they're large not
because the endpoint is rare, but because the efficacy you can have is so low.
And
in all of these trial size and the duration are somewhat fungible, but the
trial has to make sense from a corporate perspective. And, frankly, neither of
those endpoints do.
So,
a couple of problems -- and I see this is the wrong presentation. Oh well.
How
is licensure of a novel pneumococcal vaccine for the elderly to be approached
in the States when there is one or, by the time we get to doing it, more
pneumococcal approved and, indeed, recommended by ACIP but there's no data from
controlled trials in U.S. elderly populations that really addresses any
endpoint and there's no consistent dataset even from observational studies on
the more common and the more feasible endpoints of clinical interest, like
pneumococcal CAP?
And
I'm sorry. That seems to be the wrong presentation. But let me just finish with
a brief statement.
We
think that we will have to consider actually looking at validating some
alternative clinical endpoints, things that can allow us to provide a
presumptive diagnoses pneumococcal community acquired pneumonia. And that if you do that, some potential
diagnostic modalities other than blood culture allow you to increase your rates
of that endpoint by five, six, seven fold. And then you are looking at feasible
trial sizes, still large but feasible.
There
is a second bomb hidden there, which Dr. Siber mentioned, that is everyone has
to agree on a definition of pneumonia.
But we have to look at the available diagnostic modalities and say what
can we do to really validate these so that they're acceptable to support
licensure of a product.
A
second set of issues comes from the fact that, no, I don't think we can do
these are placebo control trials, at least not in the United States. There are
probably plenty of places that we can do them.
But if so, we have to think about in advance what the body of bridging
immunogenicity data to bring them back into the United States really is.
Whether it requires a functional assay, whether it requires a rebuilding 20
years worth of work in opsonophagocytic assays but this time targeting and
optomizing those assays for a protein antigen.
And
last but not least, whether we will have to eventually do trials in the United
States one way or another in which we go head-to-head with a 23-valent
polysaccharide. We, frankly, would find
that hard to justify giving that there's virtually zero consistent evidence of
efficacy of that product for a CAP endpoint.
So
I think that these are some issues that we would like to put before the
Committee in discussing not the problems of how to license a vaccine for the
elderly based on immunogenicity, but rather how can we make it feasible to do
efficacy studies in this population.
Thanks.
CHAIR
OVERTURF: Questions, comments? Dr. McInnes?
DR.
McINNES: Mr. Chairman, is it
permissible to address a question to a previous speaker right now?
CHAIR
OVERTURF: Yes, there's a moment. Yes.
DR.
McINNES: I'm wrestling a little bit
with what I think is a very beautiful paper from the PI Fry, the first author
and this model developed looking at what sorts of reduction in disease you
might get by looking at the 23-valent versus the conjugate pediatric formula
versus 9-valent and 11-valent, etcetera.
And, admittedly, the paper is published in 2002 and was looking at
serotype incidents at that time in order to give proportional rates that you
could expect for those particular serotypes that you might impact on.
I
think if I look at those data, which really the disease reduction attributable
to the 23-valent polysaccharide model looks very much like the 7-valent
pediatric with slight increments as you start to add serotypes through the
conjugate. The problem has come in with
some of this increased disease being seen with different serotypes than were
seen back in the early 2000s, and in particular the concern about 19A and
perhaps some other serotypes.
Coupled
together with the discomfort that some are expressing that for the non-inferiority
purposes who they seem to be uncomfortable about not having an equivalent
number of serotypes for this new candidate versus what the previous licensure
was based on. So I'd like to find out
from the manufacturers how flexible they feel they could be to respond to the
need for a changing formulate as the epidemiology might suggest certain
serotypes are becoming more prominent?
And I'm not suggesting that we have an annual X science like we do
influenza, but what would be the feasibility of having some flexibility that
could respond to needs for changes in formulation of a conjugate?
CHAIR
OVERTURF: Any takers?
DR.
POOLMAN: You want your name?
CHAIR
OVERTURF: We know your name, Dr.
Poolman.
DR.
POOLMAN: So far we've been thinking
more about adding serotypes and we have the experience with the 10-valent
pediatric conjugate vaccine. And with
respect to the adult situation, we're thinking more currently in the concept of
adding serotypes. But we don't know how
many. But we currently are not thinking
in the context of 23-valent conjugate.
And
what if we would have something somewhere in the middle, and there is a need at
that stage, I would say, let's wait and see. If you are in the range of 13, 14,
15 the difference with 23-valent becomes not that big anymore. And the major differences in immune
responses are so significant I'd have a hard time thinking that it's actually
not going to perform better. But if one particular serotype then dramatically
stands up and becomes a major relevant serotype and it's not an existing
vaccine, yes, we will add it.
DR.
SIBER: Pamela, you're posing a very
important question because it will be an ongoing concern, not only over time
but to address different serotypes needs in different countries. And I think
it's a question not just for manufacturers but for manufacturers and regulators
together.
Right
now the average development time for a vaccine is 12 years. And many of us are struggling to shorten
that time, but we certainly aren't going to shorten it to one or two years in
any reasonable time frame that we have before us. And some of these things are
now on a course of now four years in the direction of pneumococcal conjugate
vaccine in children.
We
have one single vaccine where we make changes on a regular basis, and we've
built it into the system. And so I
think a question your posing is, is there a way for us together with regulators
to find a path picking from a menu and not having a 12 year development plan
with all the attendant safety and non-inferiority da, da, da, da to be able to
reformulate it, especially unless one has more experience with conjugates as we
have now.
CHAIR
OVERTURF: Dr. Word?
MEMBER
WORD: I guess just on that note when
you talked about trying to reformulate it, the question then I'd come back to
is if the Committee is struggling with looking at non-inferiority, what happens
if you want to add a serotype that isn't in one that's currently there, then
how is the Committee going to determine that?
I mean, if efficacy trials can't be done now because it's too many, it
would be challenging and almost impossible then if you say yes, we could
probably substitute, but then if it wasn't in the 23-valent before, then how
are you going to make that decision? I
don't know if it's something to think about.
CHAIR
OVERTURF: No, I think it actually it
bridges on some of the questions that we're talking about today, although I
don't really find -- I guess I'm opening up the discussion a little bit. I don't really find a problem with comparing
only a portion of serotypes for immunogenicity and equivalency that overlap
that a portion of a licensed product.
And I think that's actually the problem we're dealing with today. But I think the question you bring up, which
is how do you deal with a new serotype that's not in a product that's currently
licensed, and that will actually bring up some new challenges.
But
it's possible that with time and if we can gain more data regarding both
surrogate antibody levels or avidity or optimization antibody we may be able to
define those things. And if we can define them by incorporating them in current
trials, it may be that future decisions regarding addition of new serotypes may
be a little bit easier.
Dr.
Self?
MEMBER
SELF: Yes, it does strike me that some
of the serotypes specific results that have been presented today would be a
reasonable path forward. Perhaps there are some different ways that that data
could be looked at and some sense of what the similarities are across serotypes
could be used to borrow strength across the serotypes that we actually have
data for.
CHAIR
OVERTURF: Dr. LaRussa?
MEMBER
LaRUSSA: Just a question for the
manufacturers. Do you have any thoughts
about whether there are technical limits to the number of serotypes you could
put in the conjugate vaccine? I mean,
is it even technically feasible to think about a 23-valent conjugate vaccine?
DR.
POOLMAN: It's hard to give the
limitation, but one of the nice things about conjugate is you much lower doses
of polysaccharide and usually you use ratios like one and one and one and two
the protein. So the total content of material is actually much lower as
compared to polysaccharide vaccine. So
from a physical perspective putting it together I think that could go up to
23. And with immune responses we have
to wait and see. There has been evidence that with an 11-valent conjugate
vaccine from colleague that that was immune interfaces, probably carrying use
suppression. We'll have to wait to see.
But physically I think it's doable.
Immunologically we'll have to investigate.
And
may I pose a question with respect to the issue of incomplete coverage as
compared to 23-valent and not making a 23-valent conjugate. One obvious
solution is to give the 23-valent after the conjugate. Then you secure that you
have the same and you do more. And in
that sense, I have a question to Matthew Moore. With respect to serotype 19A coming up is there a difference in
the elderly that were recently immunized with 23-valent, do you have the
information of that or is it different in nonimmunized or immunized the
elderly?
DR.
MOORE: Unfortunately, again, I have to
say the short answer is I don't know.
From the routine surveillance data it's difficult to rely on the
vaccination information that we have.
Because, as you know, adults can be vaccinated in lots of different
places and that information is not always readily available from the medical
chart.
We
are in the process of finishing up a study where we may be able to look at that
sort of information, but we're not there yet.
DR.
POOLMAN: I think it's crucial
information, it's the currently most relevant serotype. And if you can prove that the existing
vaccine is still working there, then the sequential immunization conjugate
first polysaccharide later will resolve questions on losing of coverage.
CHAIR
OVERTURF: Dr. Markovitz?
MEMBER
MARKOVITZ: Yes. Isn't it highly
unlikely that we'll be able to coordinate those events so that the vaccines are
made by two different companies or three different companies, or whatever, that
we'd actually be able to give the 23 and then -- I'm sorry. Give the conjugate and then later give the
23? How would you think that would get
coordinated in the public?
DR.
POOLMAN: I think similar situations
exist in pediatric scheduling with different manufacturers where you have
boostings with different compositions of vaccine. I don't think that should pose any issue.
MEMBER
MARKOVITZ: Traditionally, with adults
it hasn't been that easy, though.
Unfortunately. And I agree it would be nice, but it's typically not that
easy with adults.
CHAIR
OVERTURF: Dr. Karron?
MEMBER
KARRON: I was just wondering about data
that we have so far perhaps from children on duration of protection from
conjugate. Because I'm wondering from
what you presented, George, you talked about the fact that once you give
polysaccharide you're sort of stuck in this hyporesponsiveness mode. So it occurs to me that if we're talking
about a sequential immunization potentially of conjugate followed by
polysaccharide, well then we should hope that the conjugate provides very long
term protection if, say, we're talking about immunizing a 65 year old who might
live for another 20 or 25 years. Because once you give the polysaccharide, then
perhaps you can't give another dose of conjugate. And I don't know if someone wants to comment.
DR.
SIBER: Ruth, you raise an interesting
question, which is once you've primed with conjugate, if you will, and give
polysaccharide will you then have again, a hyporesponsive problem? It's actually not something that we've
looked at and probably it deserves to be looked at.
The
matter of duration of protection with conjugate themselves, we actually have in
children very good data now for prolonged protection from conjugate. I think the ABC data show that, the Finnish
with titus media study actually shows a very substantial protection for titus
media over a long period of time, up to five years. But in adults, of course, we don't have any data at this time and
that will have to be monitored closely in use.
And I think what you're suggesting is we probably should look at whether
polysaccharide after a conjugate has some form of hyporesponsiveness inducing
effect as well.
CHAIR
OVERTURF: George, I'd for you to
address one additional question. It
seems to me that you bring up actually almost an ethical question about whether
you could use non-inferiority comparisons to polysaccharides in adults, whether
you think it's ethically responsible to continue to give polysaccharides,
whether there is sufficient data to suggest that perhaps we shouldn't be giving
polysaccharide to adults and whether that can continue to be one arm in a study
in which you may be subjecting a group of adults to hyporesponsiveness?
DR.
SIBER: Gee, I don't think it's quite
that bad. Only because, you know, look
at the data for polysaccharide vaccine itself.
You have solid efficacy for five years, continued efficacy for a period
of time, albeit waning. And there's no
question about the efficacy of polysaccharide vaccine, in my opinion. So to say that it suddenly becomes unethical
to use it based on our immunologic observations I think would be taking this
too far.
CHAIR
OVERTURF: Dr. Word?
MEMBER
WORD: Just to follow-up something that
Ruth said. You know, she was talking about adults living longer and receiving
the vaccine sequentially. I was
thinking about in the pediatric population, they're high risk children that
they get a dose of conjugate and then they get a dose of the
polysaccharide. And they're going to
live a long time. So then have you
looked at that? Has anybody looked at that? Are you thinking about looking at it?
DR.
POOLMAN: There are some nice studies
published with meningococcal C, which is a good example of a polysaccharide,
and it uses hyporesponsiveness. And a British study group from Oxford did
rather complex studies of polysaccharide, polysaccharide or conjugate
polysaccharide. And the essence message
is you can -- you come with conjugate, you come with polysaccharide; you
couldn't reduce some level of hyporesponsiveness. If you come back with
conjugate, you resolve it again. That
was, I think, my take on message from these complex studies.
And
I agree with George, the hyporesponsiveness is there but it's not something
that should withheld of a polysaccharide vaccine. And there are ways to resolve it, as has been shown with
meningococcal C conjugate.
You
should not give the polysaccharide twice.
I think that's what we reaching to that conclusion.
CHAIR
OVERTURF: I think we'll proceed to the
presentation of the FDA questions.
DR.
GRUBER: My name is Marion Gruber. I'm
with the Office of Vaccines, Research and Review.
And,
Mr. Chair, with your permission before I'm going ahead and restate the
discussion points that I presented to the Committee this morning, I would like
to make a few remarks to the Committee or the Office of Vaccines, Research and
Review would like to make a few remarks to the Committee. Remarks that are unprepared and were not
rehearsed, but we felt that it is important to make these points before we get
into the discussion points, the presentation of the discussion points.
The
subject of defining for licensure and defining licensure criteria for new
generation pneumococcal vaccines to prevent pneumococcal disease has been a
difficult subject to address, not only for infant indications or pneumococcal
vaccines for infant indications, but also for the adult indication. And it has been a subject that kept the FDA,
the Agency very busy. We had a lot of discussions, meetings with the vaccine
manufactures. And we have been
discussing these issues that you have been hearing this morning for a number of
years.
And
as you heard or have heard, the issues are issues are very complex. They're very difficult, not only looking at
the difficulties to perform clinical endpoint efficacy studies, diagnostic
criteria, clinical endpoints, sample sizes but also, if you will, some of the
uncertainties that surround inferring efficacy based on a immune criteria. So
the discussions you've heard today really summed up discussions that we had for
some of the manufacturers over the last two years, at least.
And
we felt that it was important at this time to approach the Committee for their
input and advice. Because we felt that
we needed an additional opinion before the Agency goes and formulates a
regulatory framework. And it appears
that the extent of the data that you have been hearing today and that have been
presented to you is the extent of the data that we need to use to base some
regulatory framework for licensure pathways for pneumococcal vaccines for the
adult indication on.
So
I would like to then restate what I said this morning, what the Agency really
would like for you to discuss today is the most appropriate pathways that you
think -- or what the most appropriate pathways for licensure for pneumococcal
vaccines are for the adult indication taking into consideration the various
vaccine types that have been discussed this morning.
Again,
there will be no request for formal vote.
But what the FDA will do is utilize the advice that we receive today
from you to formulate a regulatory framework for pathways to licensure for
pneumococcal vaccines for adults. And I
would like to proceed now with the discussion points.
Number
one: Please discuss whether
non-inferiority immune response studies comparing a new pneumococcal conjugate
vaccine to the license 23-valent pneumococcal vaccine PNEUMOVAX 23 for common
serotypes can be used in lieu of clinical endpoint efficacy studies to support
the approval of an indication for the prevention of pneumococcal disease in
adults.
1A: If non-inferiority immune response studies
are considered sufficient to infer efficacy, please identify the appropriate
immunological parameters for use in such studies.
1B: If clinical endpoint efficacy studies are
considered necessary to support licensure of the new pneumococcal conjugate
vaccine for prevention of pneumococcal disease in adults, please discuss the
appropriate target populations and endpoints for the study.
1C: Please discuss what additional data should
be requested to support approval of an adult indication for a new pneumococcal
conjugate vaccine that would contain a subset of the serotypes contained in
PNEUMOVAX 23.
Discussion
point number 2: Please discuss what
studies would be necessary to support licensure of pneumococcal vaccines
directed against noncapsular pneumococcal antigens for the prevention of
pneumococcal disease in adults.
And
finally 3: Please discuss other
possible approaches to support approval of pneumococcal vaccines for the
prevention of pneumococcal disease in adults.
Thank
you very much.
CHAIR
OVERTURF: So the Committee members have
15 minutes to come up with those answers.
We'll
convene at 25 minutes after 3:00. Thanks.
(Whereupon,
at 3:15 p.m. the Committee recessed until 3:30 p.m.)
CHAIR
OVERTURF: I think all the Committee
members have -- there will not be a formal vote on these questions, but what
CBER and the FDA needs is our discussion on tape so they can prepare a
transcript that will actually help them develop policy.
So
I think the best way to do this is the way we did it yesterday, which was to go
around and get everybody's comments and to try to address the three questions
and the subquestions for number one.
so,
Dr. Wharton, could I start with you?
DR.
WHARTON: Sure. I think the way I see this is very much
colored by the really striking information in the background papers that
apparently the indirect benefits of using pneumococcal conjugate vaccine in
children among the elderly exceed the directed benefits of using the
pneumococcal polysaccharide vaccine in that same target population. And if we
want to do something about pneumococcal disease in adults, we clearly need a
more effective tool than we currently have.
And certainly the conjugate vaccines appear to be very promising.
That
said, we still need an appropriate body of data to support their licensure even
under accelerated approval. And I'm
uncomfortable with relying only on immunogenicity to do that, even under an
accelerated approval scenario where subsequent studies would follow. It's too unclear to me what OPA activity
actually means in an old person who may have impaired phagocyte function and
all kinds of other things going on that are key components of the immune
response.
So
although the data that have been presented on the immunological correlate are
interesting and clearly deserve further study, I'm not sure I'm comfortable
going with that for licensure.
That
said, the clinical trial scenarios that have been presented as daunting. And it's difficult to imagine some of them
being feasible to perform. One
discussion that we haven't had here is to what degree the polysaccharide
vaccine is the standard of care in European countries where we commonly perform
clinical trials, and perhaps a study among the elderly could be performed in
Europe that would not require use of a polysaccharide as a comparator. But they're difficult to think about how
those trials would actually work prelicensure.
So
I want to go back to the issue that Dr. Farley raised earlier about carriage
studies. If the prevalence of carriage
in elderly persons who don't have contact with children is in the range of one
to five percent, which is approximately Dr. Siber said, presumably it is higher
among elderly persons who do have contact with children. And so the question
that I think deserves some reflection is given that that is a highly specific
endpoint, albeit not one that has clinical benefit to the person who is not
carrying the organism, it presumably is an intermediate step in development of
disease being colonized. And so is this something that warrants the exploration,
at least as a first step, in accelerated approval that could then be followed
up with the sort of very elegant study that Dr. Jackson and others have done
using managed care database post-licensure.
So
that's my thinking on the issue of licensure of a pneumococcal conjugate
vaccine for use in the elderly.
As
far as what additional data should be needed to support approval -- oh, and
another advantage I think of looking at carriages we assume it wouldn't be
impacted by prior vaccination with the polysaccharide vaccine. So that's another bit of noise that would
fall out if we took that approach.
Clearly
I think it is necessary to have information on subsequent vaccination after use
of it with the polysaccharide vaccine after a conjugate vaccine to make sure
that there maintains the ability to add those additional serotypes if the
conjugate vaccine doesn't contain all of them, which we don't expect it to.
In
terms of what studies would be needed to support licensure of the pneumococcal
vaccines directed against noncapsular pneumococcal antigens, I don't know
enough about how these vaccines would work to know if something like carriage
even makes any sense. I don't know that.
It may be essential for that type of vaccine to do an efficacy study
pre-licensure. But I don't know. I don't know if there's alternatives that
would make sense to use.
And
as far as other approaches, again, I think it's worth thinking about studies in
populations where use of the pneumococcal polysaccharide vaccine isn't the
standard of care among the elderly where the rates are higher to see if
clinical trials might be feasible in those settings.
CHAIR
OVERTURF: Dr. Self?
MEMBER
SELF: So for the first, I guess I'd
split this up into two pieces. One has to do with the use of an immune response
as a correlate. The other has to do with its use as non-inferiority.
There
are fairly specific criteria for the use of immune response and responses in
this way, and I actually don't see that direct empirical evidence connecting it
in this case in OPA or ELISA to protection in the target populations. And so
it's hard for me to see that that would be -- there's a clear basis for using
that here.
There
are other types of arguments that seem to me to build a strong case for it being
a possible correlate of protection, but that's a somewhat lower bar. And I find the argument of well what else
could it be if it's not OPA not particular compelling. I mean, I think this is a case where we, to
quote somebody I'd rather not quote, "we don't know what we don't
know." And that's difficult for me
to get over.
So
I would be very much wanting to avoid the use of that measure as an indicator
of licensure.
So
that brings the issue to the other clause, the other types of criteria where this
could be used, and that has to do with trial feasibility. Now cases were made that standard trial
designs, efficacy trial designs would not be feasible to conduct, and there are
all the problems laid out about endpoints and the rates of those endpoints int
he various target populations. I
honestly can't tell from the discussion that we've had today and reading the
papers what the answer is, whether there is truly not a feasible way to do a
clinical endpoint study. And so it's
hard to say right now whether that kind of trumps my reservations about the use
of immune correlates.
My
best recommendation, I suppose, about this would be to have some sort of
exercise performed that would involve a number of people from the Agency and
maybe beyond to talk about a little more creative designs that might be used,
perhaps designs that would capture both direct as well as indirect
effects. And try and come up with some
wisdom at the end of a more detailed exercise that everybody joins in, perhaps,
together.
So
at the end of that, it's my turnout that this is not something that is
feasible. And then you are sort of
forced to return to these immune response measurements. Even at the end of that trail I have serious
problems just with the issues of the valiancy.
So I can't think of any way right now to calibrate the potential
increase in efficacy that might come from the common serotypes with the lack of
coverage for the serotypes that are not included in the new vaccine. And somehow that has to be addressed.
You know, one thing that's completely
clear in my mind is that the non-equivalence based on just the set of common
serotypes is not good enough as the basis for licensure. So there has to be something more to the argument
than what we've seen today, at least in my opinion.
I
think I will also pass on the question about noncapsular pneumococcal
antigens. And I think my comments I
hope at least glanced to question 3 about other approaches to support approval.
CHAIR
OVERTURF: Dr. Jackson?
DR.
JACKSON: Well, I agree that there are a
number of dilemmas. One is that giving
a lower valiancy conjugate vaccine inherently has a disadvantage in comparison
to giving the 23-valent polysaccharide vaccine. So the non-inferiority immune response criteria runs into some
problems in that regard.
I
would say that if we're looking at age groups and population groups for whom no
pneumococcal vaccine is currently recommended, then if you were to establish
non-inferiority to a vaccine that we believe is effective in some groups, that
group would then be benefitting. So,
for example, people 50 to 64 who don't have chronic conditions that are an
indication for vaccination currently, perhaps a non-inferiority approach would
be sufficient to say that those persons could receive a conjugate vaccine. In other groups, however, you're trading off
the current standard, which is to give the 23-valent polysaccharide versus a
new approach, which would be to give the conjugate, and it's the difference
between the sera group coverage that potentially puts those people at higher
risk of pneumococcal disease in general.
And so then risk would have to be balanced off against some other
advantage. And the advantage could be
that there's a higher protection against the sera groups in common to both
vaccines that the increased effective of the conjugate vaccine to sera groups
in the conjugate vaccine itself would outweigh a decrease in total number of
sera groups, potentially, or that there's an expanded spectrum of coverage of
disease protection against community acquired pneumonia for example or that
there's an expanded duration of protection. However, I don't think that any of
those advantages can be proven with a non-inferiority immunologic approach,
which is the crux on the dilemma.
On
the hand, I think that most of us or all of us want a better pneumococcal
vaccine for adults. On the other hand,
what should be the standard proof that would be required for licensure of a new
product that in most cases would probably be used instead of the current
standard of care?
So
that does run into the very real issues of feasibility of clinical trials that
we've been discussing today. There are perhaps some assumptions that could be
questioned that might allow for more reasonable sample sizes. And one would be whether hyporesponsiveness
induced to the polysaccharide persists forever or for a very long period of
time. Because if it doesn't, then you
could enroll people that receive the vaccine at age 65 and who are now 75 or
whatever, beyond the period in which you'd expect any effect, positive or
negative, of previous vaccination to now have been resolved. And in that case
you could ethically do a placebo controlled trial in which you randomized
persons to conjugate or protein or whatever type of vaccine or placebo. And you also have the advantage of higher
disease rates the older population group you study, both for invasive disease
and for community require pneumonia or specifically for pneumococcal
pneumonia. The disease rates are still not
really high, though. So, I mean, there
would still be very real issues of sample size and feasibility.
Let's
see, moving to the appropriate immunologic parameter that could be used in
non-inferiority approached. I don't know.
I would suspect OPA at some level that's considered reasonable
indications there is true opsonic activity, I don't think we would need to
prove higher levels. But just a threshold established which would then be met
for the sera groups included in the vaccine would be sufficient.
If
clinical endpoint studies are considered necessary, again I said perhaps the
older end of the spectrum of previously vaccinated persons that was considered
to be a feasible approach could be used for conjugate approaching vaccine
studies.
Additional
data, I'm sure who would pursue this.
But it seems like this issue of hyporesponsiveness to the polysaccharide
vaccine is important in considering the relative benefit of the use of
alternate vaccine strategy. And so
maybe we need to know more about that. Although certainly it seems well
demonstrated that you get a decreased antibody response to a subsequent dose of
polysaccharide given within one or five or possibly longer years, I'm not aware
of any clinical data that would suggest of putting those persons at risk of
actual increase in disease. I mean, if
we don't know the threshold correlate of protection, we don't know whether
lower antibody has any meaning or not, although intuitively we would be
concerned about that.
For
noncapsular antigens, I think as has been discussed some sort of efficacy trial
would be required for that. And other
approaches, post-licensure work will be important and the major questions then
is what degree of pre-licensure data and evidence are required to get to the
post-licensure stage.
MEMBER
KARRON: I guess I'd first like to echo
what Dr. Wharton said in terms of our sense that we need a better vaccine for
the elderly. I was struck in listening
to all the discussions today that on the one hand we don't want to set the bar
so high that we actually discourage companies from pursuing this goal. And I'm actually concerned about that. I'm
concerned that if we mandate efficacy studies, for example, that certain
individuals may decide to pursue this and that we will be left with exactly the
vaccine that we have for the elderly right now, and that is a concern for me.
On
the other hand, I think the other thing that -- the difficulty that all of us
are having is this issue of an existing 23-valent vaccine and thinking about
other conjugate vaccines of some lower valiancy number. I think we heard from Dr. Moore today that
this issue of replacement phenomena is sort
of a moving target. We don't
exactly know where we are or where we'll be with that. I do think that still, though, in terms of
looking at the numbers thus far the numbers are relatively small. But that this is making a fairly small
contribution to the overall disease burden.
I
guess I would like to dissent a bit and open the door to the possibility of
some non-inferiority studies looking just with invasive bacterial disease as endpoint. I certainly don't think that you could do that for community
acquired pneumonia. But I would want to
think about that for a conjugate vaccine.
I
think that we do need to think about at this point using a conjugate vaccine in
conjunction with the 23-valent vaccine. And so I would like to see additional
studies, as we've discussed earlier, of a conjugate vaccine followed by a
23-valent vaccine and looking at duration of protection and then looking at
what happens if you in fact come back with a conjugate vaccine again. Do you
just giving the 23-valent vaccine induce hyporesponsiveness?
I
guess sort of an answer to the question 1A about the appropriate immunological
parameter, I think OPA is probably the best that we have to look at that.
I
guess the other comment that I would like to make is that as we consider
studies and we think about target populations, we shouldn't just think about --
I feel very strongly that we should not
look at surrogate populations for the elderly, we should look at the elderly.
So we should not be doing studies in 50 to 65 year olds. We should be doing studies in those over 65. And I think also among those over 65, we
need to look at a range of ages. So we
need to look at the elderly. And I
think we need to look at the very elderly.
And
the only other comment I think I'd like
to make, which I think is clear from what other people have said, is that in
terms of thinking about non-capsular pneumococcal antigens, then clearly I
think we do need efficacy trials.
CHAIR
OVERTURF: Dr. Piantadosi?
DR.
PIANTADOSI: Thank you. My comments are not structured in the same
way as the questions, but I'll go through them and I think I'll cover most of
the important points.
In
my judgment the essential problem at the heart of the FDA questions regarding
development of new vaccine for pneumococcal pneumonia is the classic debate
about validity of surrogate outcomes.
In this case OPA is the proposed surrogate. And the question is whether
or not it can substitute for definitive clinical outcomes in vaccine
development, such as clinical pneumonia attributed to pneumococcus or invasive
disease.
The
questions surrounding OPA are made somewhat difficult by it being a laboratory
measure, however well standardized, rather than a surrogate clinical
outcome. Guidance on this classic
question is abundant in the methodologic literature. The validity of OPA as a surrogate for prevention does not depend
on the information presented today.
For
example, it is not definitively valid because it seems to measure a vital
component of the immunological response to established infection or because it
is statistically correlated with other immunological measures. Nor would it be valid even if it were
correlated with a definitive clinical outcome.
The
validity of OPA as a surrogate depends on its tracking direction and relative
magnitude, the same way as the definitive prevention outcome after
vaccination. This is basically the
Prentice criterion applies in this context.
No data with this strength of evidence or quality have been presented
here today.
The
difficulties with OPA are illustrated in a couple of its characteristics. It
does not appear to correlate quantatively with clinical outcomes in
adults. Even if endorsed for
polysaccharide vaccines it would be irrelevant for protein constructs. Thus, OPA has not minimal standards for a
surrogate outcome.
With
regard to non-inferiority my opinion is that the difficulties of quantitative
interpretation make OPA especially ill-suited to design an interpretation of
those kinds of trials.
OPA
is an appropriate outcome on which to base developmental decisions and can be
used to increase the reliability of developmental choices and reduce the risk
of failed comparative trial.
I
am also concerned and sympathetic to the potential problems of doing large
randomized trials in prevention, and this context seems particularly difficult
because of issues such as bacterial subtypes, difficult diagnostic criteria and
incomplete efficacy. But such problems
are not cured by doing smaller trials with a potentially invalid outcome.
Another
potential problem in the future from such an approach is having economic and
ethical imperatives, perhaps wrongly, established for suboptimal treatments by
our health care system. This can make
clean definitive studies more difficult for new preventives and therapeutics.
I
would close by mentioning a couple of ideas that have not come out in today's
discussion, but that might make adequate and well controlled studies more
achievable.
In
the presence of a relatively safe intervention, as vaccines seems likely to be,
it makes sense to relax the type 1 error in our study designs. This would be
breaking ground for the FDA, but it's appropriate to set such criteria to
reflect the consequences of making the respective error. For example, for a safe intervention a type
1 error rate of, say, 10 percent or higher might be appropriate and would help
reduce the size of the studies needed.
The
FDA and sponsors should also consider alternatives to the standard designs that
were displayed today, mostly for their seeming lack of feasibility. I'll
mention three possibilities, not because I know them to be appropriate in this
context, but to try to broaden the thinking and discussion about study design
and methodology.
First
are cluster randomized designs where although the total sample size of
individuals would be large or larger than those mentioned, the logistics of the
trial might be more manageable than individual randomizations. Units of randomization might be taken to be
residence homes, group practices or even entire cities for example. These are the kinds of trials that have
historically been applied in developing countries to investigate prevention
interventions.
Second,
some consideration might be given to factorial designs constructed in a way to
use their potential efficiencies.
Pairing the pneumococcal vaccine question with another prevention
question, for example, might make for more active participation by adults and
practitioners alike. I think it's important to note that factorial designs are
not always more efficient, but when designed properly you can get a two to one
efficiency.
Finally,
single cohort designs with definitive outcomes may have a role here as
well. They can in principle provide the
kind of evidence needed and would be made more reliable by the CDC surveillance
data that we were shown earlier.
Thank
you.
CHAIR
OVERTURF: Dr. Steinhoff?
DR.
STEINHOFF: I agree with many of the
comments made. I'll just reiterate some
of them and add a few points.
I
think with regard to the first question about non-inferiority as a way of
moving forward, it seems to me that aside from the point of fewer serotypes,
which is a major point, there's no reason not to use that criteria to license a
conjugate vaccine. We've heard there's
historical precedent for doing that.
And if it can make as much antibody of whatever type as an existing
vaccine, even though the overall serotypes coverage is less, it would seem to
me that's something one could still do.
It leads for implications for what you do after you license such a
vaccine, because if it is in fact more effective on fewer serotypes, the
overall impact might be greater.
The
other point, though, with regards to non-inferiority, that would apply only to
the connection that we've heard about, which is the vaccine is immunogenetic to
some extent in adults and has an effect on IPD, culture positive disease. I don't think that the similar reasoning
would apply to community acquired pneumonia where we don't have a similar
confidence that the vaccine is making a difference.
So
for similar indications and similar antibodies, it seems to me that is
something one could consider.
You
are still stuck with the problem of fewer serotypes. So one would have to postulate that there's a greater effect.
In
terms of which test to use, which is part 1A, I find it very troubling that the
effectiveness of antibodies is so different related to age groups. And some of the suggestions made about
comparing OPA titers with adults who have received the currently licensed
vaccine as a way of measuring non-inferiority makes sense. We don't have anything else right now,
unless we do an efficacy trial.
To
go on to the second point about if an efficacy trial is done, it seems to me
that that trial should consider something which wasn't discussed very much
here, is to think about better diagnostic technologies to define what might be
pneumococcal disease beyond the blood culture criteria that we've used.
We
heard a little bit about looking for antigen in urine. And there are at least two ways of doing
that, both of which I suspect could be refined. That would take, though, a fair amount of development work before
you start the efficacy trial.
I
think that the category of punitive pneumococcal disease or possible
pneumococcal disease which would include a clear clinical definition with a
variety of other criteria such as antigen detected in urine or blood maybe some
markers of inflation, and of course some kind of an x-ray finding might give
you a better indication of what disease you're preventing, even if it's
somewhat insensitive or even nonspecific.
My guess is that given these kinds of criteria you could show an effect
of a pneumococcal vaccine in overall CAP rates because you're focusing on
what's more likely to be new.
I
mentioned the crucial issue if you don't have the same number of serotypes how
much can you rely other criteria.
I
agree with the points that others have made regarding the non-capsular
pneumococcal antigens that to license those I think you do need to have an
efficacy trial. Those should be planned
so that one could begin to look at the information regarding antibody levels
that appear to be protective, looking at the kinds of graphs and charts we saw
today. I think that could be done right at the beginning to get some
indication.
Those
studies, too, by the way would benefit from the category of punitive
pneumococcal disease as one of their endpoints.
That's
my comments. Thanks.
CHAIR
OVERTURF: Dr. Word?
MEMBER
WORD: I think the easiest thing, in one
sense which I think probably everybody's in agreement is, is looking at the
pneumococcal vaccine directed against the pneumococcal antigens. And actually the way to go with that would
be efficacy trials. I just find the
whole concept very exciting and would look forward to seeing that move forward.
In
terms of just going, looking at surrogate markers. You know, originally I was really excited about it, I thought
this would be good. And then as I
listened a little more, I started saying you're telling me this vaccine is not
as protective in elderly people yet you want me to say that okay, I can compare
it to something that doesn't work so well.
And, okay, maybe it won't be inferior but is it the best thing because
they have a hypoimmune response. Then,
you know, looking at this OPA, which I learned a lot about during this time
period here. I said well I'm hearing
that there's differences in terms of age groups and how people respond, so it
might be nice to see if you break down the ages. There's something that happens at 65, well happens at 64? What's going on between the person between
50 and 64 years of age? Maybe I want to
know what the normal is there. Maybe I
want to know in a few age groups.
Because people do live longer now.
People are living 80, 90 years of age and it would be interesting just to
see. And I think it could potentially
be a correlate and something that people can look at.
Right
now I'm not convinced because I'm not quite sure how to interpret it, and so
I'm not as comfortable with it. Even
though I'm not so thrilled by the non-inferiority with using less pneumococcal
serotypes, I think if the companies had approached the conjugate vaccine with
the 23-valent, it probably would have been more supportive of it because it
probably would have been my own comfort level more than anything else.
And
I guess I'll stop there because I don't really know what else I want to
say. I've actually agreed with a lot of
other things that were said, there's no need to repeat it.
CHAIR
OVERTURF: Dr. LaRussa?
MEMBER
LaRUSSA: Okay. I'll just go down the list.
I
think the first thing is if you want to have a really big impact on the
pneumococcal burden, the idea of improving the pediatric vaccine should go near
the top of the list.
As
far as the first question whether non-inferiority immune response studies can
be used in lieu of clinical endpoints, efficacy studies at least at this point
in my opinion is no. I think it's possible to design trials,
and I'll talk a little bit more about that in a second.
In
terms of what the appropriate immunologic parameters to look at, I'd like to
hear more about the OPA assays, especially in the age groups we talked about
with the appropriate controls. And I think the idea of looking at changes in
colonization rates is really an intriguing way to look at a second parameters
and may, in fact, answer some of the questions that we've had.
As
far as the part B if clinical endpoint efficacy studies are necessary, I think
we do need to look in adults over the age of 65 and come up with a reasonable
definition of pneumococcal pneumonia, and I think that's possible. I think we
can do chest x-ray plus some sort of urinary antigen. It's not going to be perfect, but I think it will be a reasonable
thing to look at.
As
far as additional studies, I think we've got to look at these combinations of
vaccines that practitioners will use, whether it's polysaccharide followed by
conjugate because there's already that population out there or conjugate
followed by polysaccharide followed by conjugate. And people are going to do that, so we need to figure out what
exactly those combinations will do.
I
think with the protein vaccines at this point we're stuck with efficacy
studies.
And
finally, in terms of additional approaches I think if we really scratch our
heads and do not come up with a reasonable efficacy study and we do end up
approving the conjugate vaccines on the bases of immunologic markers, then I
think that approval has to be contingent on rereview once the large databases
give us the answer about whether they've had some impact on community acquired
pneumonia.
CHAIR
OVERTURF: I largely agree with what's
been said. I will say that clearly you can use immune studies in part on
non-inferiority basis for licensure of new vaccines.
One
thing it seems to me that hasn't been -- and I didn't hear any data to convince
me that we know enough about the optimization assay, that can be used solely as
even a single immunologic correlate. I
think it probably has to be combined with things that we do understand a little
better, antibodies despite we don't understand all the quality about that
antibody.
There
was a point made about a carriage and we heard repeatedly that carriage rates
in those who have low exposures to children are low. They're certainly not what we see in children, but they're
certainly much higher than disease rates.
And it would seem to be an additional part of what should be added and
was clearly one of the benefits and one of the additional benefits we're
already seeing with conjugate vaccine use in children. So it seems to me folly
not to include carriage studies as one endpoint for evaluating conjugate
vaccines even comparing them against polysaccharide vaccines.
And
I would echo what a lot of people have said about the problems with dealing
with a 9 or 11-valent vaccine and a 23 vaccine. And with an appropriate selection of the serotypes based on
current epidemiology you could reduce the difference in potential efficacy
between a polysaccharide and a conjugate vaccine to a very small number with
perhaps only the addition of another, what, 3 or 4 serotypes. Because the actual number of potential
coverage that you'd get with some of the additional serotypes only come up to 4
or 5 or 6 percent total. So I think some real concern needs to be thinking
about adding some serotypes that come closer to matching the coverage or at
least the minimizing the differences in coverage between the two vaccines.
I
agree with Dr. LaRussa that I think there can be better standards set for
diagnoses of community acquire pneumonia.
And somebody made the comment that it is more difficult in adults than
it is in children. I feel just the opposite. Actually it's easier. Actually low bar pneumonia is actually a
much easier radiographic endpoint to define in adults than it is in children,
particularly if you will go the population that's at most risk for those, which
was the population we are most interested in, which somebody commented on,
which were the very elderly population.
Actually,
that was done in the Kaiser trial on children, the ability to predict efficacy
against pneumonia began to rise as the specificity occurred. The problem in
children is that you're dealing with a lot of viral disease, which is not going
to be effected radiographically by the introduction of a pneumococcal
vaccine. But it is also possible.
I
think I would be satisfied if we had a narrow enough gap, we showed striking
effect on carriage because that's actually the first step in the pathogens to
disease to licensing a vaccine provided there were very, very, very strict
concepts of what had to be done with phase for efficacy trials. So that one could rapidly perhaps get an
answer once a vaccine was licensed.
It
may be, you know if we're really talking about studies regardless of some of
the manipulations that Dr. Piantadosi mentioned, I still think that we would
have very, very large trials. But we
are getting to the point where we are accepting trials some 60 and 70,000 in
other vaccine trials now that we are doing.
So that some of these I do think have a feasibility.
For
the non-capsular serotypes I think
you're stuck with some kind of efficacy trial.
One
thing I didn't hear from those, and I assume there is no effect on carriage and
so I don't think carriage would be an option in that particular kind of a
trial, but it would be interesting to know.
Dr.
Robinson?
DR.
ROBINSON: The first thing struck me was
what Dr. Moore presented and are we moving down a pathway in which a very good
vaccine for infants and young people is driving the pathogen and the disease
that it causes to be this phenomena of capsular switching and that are we going
to see prevalence of antibiotic
resistent strains or subtypes and then also to have it be even more
invasive I think that's just something
that has to be watched in the future.
But if this is the paradigm of where you give a capsular vaccine first
followed at some interval later on with a polysaccharide vaccine, then what is
going to be that interval? And then
what's going to be happening during that interval especially if you say you
give it to adults, which is what we were asked to address, at 50 years old
followed by how many years later? Well,
we saw data that it looked like three years from a Finnish study. That may be the same type of efficacy. But what if it's not until you're 65? And then we're having the infant programs
that are actually driving certain subtypes to be more prevalent and more disease
causing? As a conceptual thing it
troubles me a little bit in how that's going to be handled.
Pragmatically
though looking at different intervals from the time you receive the first
immunization primarily with a capsular vaccine followed either another capsular
vaccine or a polysaccharide vaccine, I think that needs to be added in these
trials.
Relative
to the protein based vaccines, I think the guidance that the FDA provides for a
true efficacy trials for a well characterized biological are in place there.
And I think that it has to move that pathway with the development of the
different diagnostic for the clinical samples.
I
would like to see more emphasis on mucosal immunity and what can be done there
to look at not only in terms of dates of IGG, but also with IGA and to see what
really impact that has and it can be done as a subgroup of one of the clinical
trials.
And
finally, just looking at where is the future for these vaccines, just looking
at what the issue is and how can you enhance the immunity in the elderly
population regardless of what vaccine you use? And to me it looks like a
vaccine and wanting some of immunostimulant, whether it be a device or an
adjuvant or some other type of immuno cytokine. And so that would be a further direction down the road.
MEMBER
PROVINCE: My remarks will be brief and
contingent upon my ability to read my own handwriting, because I've been
jotting down notes here.
Speaking
as a consumer representative, as I am on this body, what consumers want of
course is safety and efficacy. And as
we've heard, of course, people are living longer and they have higher
expectations for their personal health. You know, I think of my aunt who is 101
years old and has lived 36 years beyond the time she would have received her
pneumococcal vaccine. She's still out
in the community living on her own, and she's not that unusual anymore. We see more and more people living to the
age of 100 and beyond and so we can't think of 65 as quite the way we would
have, perhaps, in previous decades.
Clearly
with all we've heard in the last couple of days we all agree, I think, that we
need something better. But as Dr. Karron mentioned, we don't want to set the
bar too high. If we do that for any vaccine, we set ourselves back, we retard
the development or potential development of new vaccines and we really need to
look at that and be cautious that while being very careful about the issues of
safety and efficacy, that we don't set the bar so high that it's just
unattainable.
I
was very interested in the illusions to creative designs to show efficacy that
was alluded to earlier as the standard efficacy trial designs could get to be
such large sample sizes that they'd be unwieldy and unfeasible, and we're
running into that more and more. So I
think we need to look at some of these strategies that have been mentioned and
take a close look at that.
I'd
like to see some additional work in giving the conjugate vaccine after the
polysaccharide vaccine, perhaps to work around the problem of the fewer
serotypes that would be included in the conjugate vaccine. And, you know, perhaps in populations where
the polysaccharide vaccine has not been used to use some data from those
populations I think would be very helpful.
And
in any event, however it ends up, I think post-licensure work -- I always feel
like a broken record because I say this almost every time I open my mouth. But I think post-licensure work is
imperative, is more and more important not only looking at efficacy, but in
looking at rare and very rare adverse events.
And with that, I'll conclude.
DR.
McINNES: I've been listening all day
and reflecting back really on the last 16 to 18 years and thinking about
everything we learned from hemophilus conjugates, polysaccharides and
conjugates, meningococcal polysaccharides and then conjugates and then the pneumococcal polysaccharides and the conjugates. And I think we have been surprised every
time about the power of this family of conjugate vaccines. And with regard to pneumonia we reflect back
on the hemophilus influenza type B conjugate trial in the Gambia and the very
surprising finding of the impact on all cause pneumonia reduction by 15 to 20
percent. It was unprecedented. We didn't anticipate it at all.
I
would say that the efficacy data from pneumococcal conjugate as evidenced by
the Kaiser trial, the otitus media trial, the South African trial, the Gambia
trial has surprised us every time how astonishingly powerful these vaccines are
in protection against not only invasive disease, but as illustrated in the
Gambia against pneumonia, against radiographically confirmed pneumonia, culture
positive pneumonia, all cause pneumonia, hospitalization visits; these are
powerful tools we have intervention.
I
don't think it's a leap of faith that the primary mechanism of host defense
against streptococcus pneumonia us antibody.
Extrapolating from that I think the functional assessment as measured
OPA assay, I think it does measure only functional antibodies. I think those are correlated with protection
against invasive pneumococcal disease.
And I am persuaded that non-inferiority immune response studies are
sufficient to infer efficacy for pneumococcal conjugate vaccine.
With
regard to the serotype coverage, I think it is very clear that this discussion
is not over, and the coverage it needs to be appropriate and it needs to be
responsive to changes in ecological -- and I think that's a little bit unusual
outside of our influenza experience, but I think maybe this is time to say
this: We have to embrace this in this discussion
if we're going to take this path. So I
think we need a new system to allow that to happen.
So
this multifactorial idea of thinking about immune response, quality of the
antibody response, the duration of the antibody response; I think it's a
compelling constellation that could be taken forward and flushed out more and
thought about. But at this point in time I'm persuaded that there could be a
path to licensure for these vaccines without clinical endpoint trial up front.
The
induction of the functional immune response that allows subsequent vaccine if
in fact it's deemed that we do need to maintain a flexible system that can give
us broader coverage, not necessarily only through the conjugate I think is very
interesting. And I think one should
look very carefully at what data we have and what data perhaps could inform
that. And when I look at the modeling
paper and taken into account that we might be able to have a system with more
flexibility, I suspect that we will have the same or better impact on invasive
pneumococcal disease and we'll gain protection against pneumonia with
integration of pneumococcal conjugates into adult vaccine and certainly into
elderly vaccine. The question is what
detection systems need to be put in place to monitor that and to inform
changing decisions if those are appropriate.
I
think that reflects my thoughts. I
don't have anything novel other than what I have heard here to contribute to
the discussion around the non-capsular pneumococcal antigens. That's it.
CHAIR
OVERTURF: Dr. Farley?
MEMBER
FARLEY: Yes. I first of all would like to just say that I think that the idea
of targeting adult populations with these conjugate vaccines for pneumococcal
disease in particular is a very high priority, and I want to do everything to
encourage this to go forward. And that
may mean that we may have to in some ways make some compromises from the
standpoint of how the process from a regulatory standpoint for licensure may be
handled.
I
would far prefer efficacy trials, and if they were to be done I would prefer
them to be really targeting pneumococcal pneumonia in whatever best way they
could target pneumococcal pneumonia within the limits of our diagnostic
capacity. But the idea that urinary
antigen may be more useful or is more useful in adults makes that a little bit
more feasible than in young children.
However, I'm fairly pragmatic and see that as a huge barrier to the
sponsor's interest in taking this forward.
And my sense is that we really will likely have to come up with
something that will be less stringent.
And because of all that has been discussed, I think that whatever we can
do to maximize the immunologic parameters and maybe adding colonization so that
it isn't just OPA, but OPA -- of whether avidity further studies are required
in some subset. And considering the use
of colonization, although it certainly can't be used as a true clinical
endpoint, but it would certainly I think be very encouraging to all of us to
see that there was a direct impact on colonization that mirrored the serotypes
in the vaccine and was similar to that seen in pediatrics.
So
I guess I'm coming around to the idea of trying to come up with a way with as
much stringency within the immunologic comparisons with perhaps colonization
added to it. And anyway that so called superiority could be demonstrated or
advantages maybe would be a better way of saying it; advantages such as the
avoidance of the hyporesponsiveness or that we actually, which we won't be able
to show, but the advantage of this might increase the level or the extent of
the disease to include pneumonia rather than just IPD would be advantageous, I
think, to the process.
I
do think the reality is that in the clinical world they're probably going to
continue to want and need and grasp on to the idea of that safety net of the
23-valent. And so at least for the
beginning of this process of having a new conjugate available for adults, I
think clinicians may still have a tendency to want to sort of top it off with the
23-valent. And for that reason the idea
of documenting the interrelationship of these two vaccines I think I also
believe would be important in the process of evaluating them in the licensure
process.
I'm,
again, very excited about some more broad based protein antigen based vaccine
of the future. And what occurs to me
besides the agreement that efficacy studies will be required is that maybe some
of these creative efficacy studies that Dr. Piantadosi was putting forth could
be also considered, because this is a daunting task to look at pneumococcal
pneumonia prevention for the protein vaccine, that maybe some creative
discussion of those approaches for the protein efficacy studies would be very
interesting. And I really think that those studies we need to take the
opportunity to show that something is preventing pneumococcal pneumonia and not
just IPD. And that would be a good
point of having the bar at that level or at least having that be a goal of the
evaluation.
And
then finally I very much agree with a very stringent post-release evaluation of
the effect of the introduction of this vaccine with studies such as Dr.
Jackson's study or the ABC's indirect cohort sorts of studies.
CHAIR
OVERTURF: I'm just going to make a
point. I'm going to have to leave
because I live in a third world state that only fly airplanes there on rare
occasions. And Dr. Markovitz will end
the discussion and take over as Chair.
Dr.
Royal?
MEMBER
ROYAL: Well, much of what I'm going to
say it may seem a bit redundant, because it's already been mentioned, but again
it is very important to develop an effective vaccine, especially in the
elderly. And, however, when it comes to choosing between an efficacy study and
a non-inferiority study, I think it's interesting that we're not using the term
equivalency study, especially since the valancy of the vaccines are not equal.
My
tendency is to lean towards supporting efficacy studies. It was mentioned earlier that there are
creative ways for designing clinical trials. There are ways of new assays that
are being developed to try to increase the sample -- the number of patients
that can be pulled into those studies.
We've heard a lot about that today. But we've heard a lot about the OPA
study. And some of that dealt with that
assay in the context of killing, which means to in fact correlate with some
efficacy for the vaccine. I think that
that should be pursued and validated further.
It
is exciting that a protein assay vaccine is being developed. Clearly one would need an efficacy trial for
that to move forward. And the newer
approaches for definitively diagnosing pneumococcal disease would be important
to employ in assaying that vaccine.
With
respect to invasive disease and whether a non-inferiority study would be
adequate for approving lower valancy vaccines for trying to prevent that type
of disease, we fall into the same sort of problem in that you end up preventing
a subset of pneumococcal disease and eventually those caused by subtypes that
aren't represented in the vaccine will start to emerge. So that issue has to be addressed
proactively whether or not it's best to do a serial immunization with the
conjugate followed by the polysaccharide or two conjugates, the first being
what's currently available and subsequently with what wasn't represented in the
previous vaccine. Whatever the decision is, we'll find ourselves here at the
table having the same discussion.
There
was very brief mention early on during this meeting about other potential
markers of response to vaccine, cytokine responses that seem to correlate at
least with OPA responses and perhaps other clinical indicators of responses to
the vaccine. When you think very little
about the mechanisms associated that underlie an effective response, we're
looking at a certain type of immune cell in the OPA and just what are some of
the factors that are associated with effective killing or in the immunized
patient with an effective response. I
haven't heard much about what those are, and I think it would be useful to be
able to get more information on that. Maybe the OPA assay might not turn out to
be quite as useful as some of the more genetic cytokine or chemotactic measures
in the context of other information.
Finally,
with respect to the populations that we'd like to see targeted with the vaccine
in the elderly, another bit of information that would have been helpful, at
least for me, would be to have known the demographics of the elderly
population, whether or not the poor responsiveness is seem among all those that
are vaccinated or whether or not there's certain subsets who tend to have a
particularly poor response, and certainly there may be unique issues that could
be targeted within those populations and that it would be important to know
about.
ACTING
CHAIR MARKOVITZ: Seth?
DR.
HETHERINGTON: I'm going to be brief
because of the time of day and restrict my comments to two topics. One was the
question about whether an immunologic assay could be performed in lieu of a
clinical trial.
I
have no doubt that antibody is protective, particularly antibody against
capsular polysaccharide. I have no
doubt that the mechanism of action is opsonophagocytosis. There are doubts, however, with the OPA
assay as described represents what happens in vivo. It used HL60 cells, the
first line of defense in the respiratory tract is the macrophage. Also it leaves open a doubt as to what
results really correlate with efficacy and has a standard really been
established, not just in the performance of the assay but the readout of the
assay.
So
I think there's -- and I've heard this going around the table, quite a bit of
discomfort about replacing a clinical trial with the OPA assay.
Second
is related, it has to trial feasibility which seems to be the primary driver
for using a surrogate marker. There is
a bit of disconnect, at least on the surface in saying, and I believe it is
true, that the pneumococcal vaccine would have a big public health impact and
then on the other hand we're saying we can't show that prior licensure. Perhaps
there's a way to find some intermediate ground, but it should be measurable in
some way as to what the public health impact is going to be. In that regard, although we don't discuss
costs here, using the numbers that I saw today about estimated attack rates and
estimated efficacy, and this could be off by an order of magnitude, but what I
find on the back of the envelop calculation is a cost to prevent one
pneumococcal infection of somewhere in excess of a million dollars. So there is
a reason to consider what the cost will be to society and whether or not we're
willing to accept an in vitro assay as a measure of potential benefit.
If
approval by an immunological assay is ultimately a path that the FDA wants to
take, then it should be perhaps under an accelerated approval mechanism by
which there are strong commitments post-marketing. And I think we've heard that
from others. To do a large enough study
to demonstrate clinical benefit and to particularly measure the impact of
replacement disease.
The
single most important lesson I learned today was that the impact of replacement
disease could oblate, if not just severely decrease the efficacy of a vaccine
long term. And I think that's something we need to address as we go forward and
consider the implementation of these vaccines across very large groups in our
population.
ACTING
CHAIR MARKOVITZ: Thank you.
I'll
go last then, and originally there were so many good points raised I think in
this discussion that I started out with the idea that I was going to quote
various people who all had made good points. But then everyone made a good
point, so I'm not going to go through everyone else's comments. But I would
like to highlight a couple of my particular concerns.
One
is I would like to echo the comments that a protein vaccine in the future which
spans the different serotypes is something very exciting. And I would not like our decisions today to
make it ultimately harder for a vaccine like that to come to market, other than
perhaps if it can raise the bar in terms of true efficacy.
Second
of all, in order to have a true non-inferiority study you have to have
something to measure. To my knowledge,
anything that's ever gone through our Committee before where non-inferiority
was accepted in terms of immunology, there was a very well characterized and
well accepted test which indicated immunity. We don't have that here with the
OPA, in spite of multiple attempts to elicit true data that really supports
this as being the test. I haven't been
able to do that in questioning the manufacturers.
I
would echo what Seth said and to some degree what Pam said, although taking a
little different spin on it, which is that I certainly agree that antibodies
are going to be utterly crucial to this process. But the question is really does this test measure those
antibodies. So I have a lot of concerns
about doing a non-inferiority immunologically based study.
And
then the second and obviously crucial point here which if it were different,
might allow us to get around some of these concerns is that we just don't have
enough serotypes. And again, in the
past when we've approved vaccines based on non-inferiority, there's never been
a drop in the number of serotypes that I'm aware of. So dropping the number of serotypes that I think is very potentially
quite dangerous now, I think as Gary noted before his departure for the third
world of New Mexico, that it is true that we might not need 23 serotypes in
there in order to have really good coverage. But I think we need more than 11
or 13. So I think that that's going to
be a very important consideration.
Lastly,
I would like to say that I am very enthusiastic ultimately about, contrary to
what it may sound like, I am very very enthusiastic about the idea of applying
conjugate technology to this issue. And
so I would like to, hopefully, see clinical studies. But if we do end up having
clinical studies, I would hope that the FDA and the manufacturers would show a
fair amount of flexibility in how those studies would be done. We might have to
rely more on studies in other countries or specific groups, or anything that is
deemed ethical. And I think a number of my colleagues have made some very good
suggestions about how to approach that.
And
so, I think that's the end of my comments.
Do
we have any other comments people need to make before we adjourn? Anything that you need to mention before we
quit?
Christine?
Okay. Meeting's adjourned. Thanks, everyone.
(Whereupon,
at 4:39 p.m. the meeting was adjourned.)