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Dispatch
Detecting Biological Warfare
Agents
Linan Song,* Soohyoun Ahn,* and David R. Walt*
*Tufts University, Medford, Massachusetts, USA
Suggested
citation for this article
We developed a fiber-optic,
microsphere-based, high-density array composed of 18 species-specific
probe microsensors to identify biological warfare agents. We simultaneously
identified multiple biological warfare agents in environmental samples
by looking at specific probe responses after hybridization and response
patterns of the multiplexed array.
Accurately detecting and identifying biological warfare agents (BWAs)
is the focal point for countering bioterrorism. Current methods used to
identify BWAs are primarily focused on a single target agent (1–10).
In contrast, the fiber-optic, microsphere-based, multiplexed arrays described
in this paper can rapidly screen and simultaneously identify multiple
potential BWAs, enabling an efficient response to a bioterrorism attack.
Such multiagent analysis is difficult because it is usually complicated
by interferences between assays and the large number of BWA probes.
We developed a platform to simultaneously detect BWAs with an array composed
of DNA probe-functionalized microspheres that are randomly distributed
onto microwells generated on the end of an etched coherent optical fiber
bundle (11,12) that contains 6,000–50,000 individual
fibers. Methods are described more fully in the Appendix.
A multiplexed array was fabricated by distributing up to 18 different
microsphere sensors into the optical fiber array with species-specific
50-mer DNA probes corresponding to 6 BWAs of interest (Bacillus anthracis,
Yersinia pestis, Francisella tularensis, Brucella melitensis,
Clostridium botulinum, and vaccinia virus) and 1 BWA simulant,
Bacillus thuringiensis kurstaki, with each organism represented
by at least 2 probe sequences (Appendix
Table 1 [ 47 KB, 1 page]). All probe sequences were designed with software by Illumina,
Inc. (San Diego, CA, USA), and the specificity of the probe sequences
was checked against GenBank by using BLAST to have minimal cross-hybridization
potential. Employing multiple probes for each BWA reduces the potential
for both false-negative and false-positive results in environmental samples.
The inherent redundancy of each probe type on the array, because each
microsphere type has many replicates, provides additional confidence in
detection and enhances the signal-to-noise ratio. Because the assembly
process for the arrays is random, each bead type is encoded with an identifying
optical bar code (11,12) created by entrapping dyes
in various combinations within microspheres, to differentiate microsphere
probe types from one another.
To ensure sensitive detection of BWAs with high accuracy, the performance
of this multiplexed, high-density array was assessed by examining
the detection limits and specificity of probes with Cy3-labeled synthetic
targets (the synthetic target is a 50-mer oligonucleotide complementary
to the probe). We modified our previous protocol of microsensor preparation
(12) by using an increased concentration of cyanuric
chloride solution in the probe activation step to achieve a more
complete and efficient coupling of DNA probes to microspheres. The
improved microsensor preparation enabled a detection limit as low
as 10 fmol/L (in 50 μL
volume) within 30 min hybridization time (data not shown). While the
probes were selected to avoid the formation of secondary structures,
such structures were not completely eliminated and probably affected
the hybridization efficiency, resulting in higher detection limits
for some probes on the array. To evaluate probe specificity, arrays
containing beads with only a single probe type were exposed sequentially
to the synthetic complementary target as well as to all noncomplementary
targets. Cross-reactions were observed between probes from the same
organism such as BA1/BA2, BA5/BA6, BTK1/BTK2, YP1/YP2, and FT1/FT2
(probes are abbreviated according to the organism from which they
were derived: BA, B. anthracis; YP, Y.
pestis; FT, F. tularensis; BM, Brucella melitensis,
CB; C. botulinum; VA, vaccinia virus; and BTK, Bacillus thuringiensis
kurstaki; details in Appendix
Table 2 [93
KB, 1 page]) because some of the sequences for each probe pair
overlapped, as probes were designed to be specific to the same target
gene of the BWA. While in some applications cross-reactions are undesirable,
in the present context the cross-reactions between probes from the
same BWA confirmed each BWA in the sample. In addition, some minor
cross-reactions between probe types from different BWAs were observed
because of sequence similarity in spite of the careful probe design
for each BWA (Appendix
Table 2 [93
KB, 1 page]). These cross-reactions could be advantageous, since
they generated a unique response pattern across all the probes on the
multiplexed array for each target BWA and provided additional information
to identify BWAs. As a result, any BWA can be simultaneously identified
with this multiplexed array by looking at the high signals resulting
from the specific response of each individual species-specific probe
as well as the response pattern across the array.
To sensitively detect target BWAs, polymerase chain reaction (PCR) was
used as an amplification step before hybridization on the multiplexed
array platform. Amplification was essential, especially when BWAs
were present at trace levels in environmental samples (see below).
Primer pairs that corresponded to each of the target sequences were
designed specifically for each BWA (Appendix
Table 1[ 47
KB, 1 page]).
Each primer pair amplified the respective BWA sequence from an autoclaved
bacterial culture (Appendix Table 3)
during asymmetric PCR. Figure 1 shows the detection
of PCR products derived from each individual primer pair based on
single bead–type arrays. The variation of the probe responses to PCR
products can be explained by the different concentrations of the autoclaved
bacterial cultures used as templates in PCR, the varying efficiency
of primer pairs, or the potential of PCR products to form secondary
structures. While carefully designed and optimized to have PCR products
with a shorter length (147–201
bp), some of the amplified PCR fragments might form secondary structures
(e.g., BA5). The formation of secondary structures makes the DNA fragments
that were complementary to the array probe sequences inaccessible
for hybridization. For these targets, the hybridization efficiency
was affected, giving low hybridization responses to PCR products.
In addition, the position of the target sequences within the PCR amplicons
could affect hybridization efficiency. Oligonucleotide probes complementary
to the middle part or the 5´ position of PCR products showed
lower hybridization efficiencies than did target sequences close to
the 3´ positions. This observation
was likely related to steric hindrance that led to less accessibility
of PCR products to the probe sequences on the array.
To assess the limit of detection with real bacterial samples, 10-fold
serial dilutions were made from the autoclaved cultures of each BWA
(Appendix
Table 3) and used for PCR followed by array hybridization (summarized
in the Table). Specificity tests of primer pairs
were performed by applying each primer pair to other nontarget bacterial
cultures individually, and no nonspecific amplifications were observed.
To investigate the ability to simultaneously detect BWAs, multiplex
PCR was used to analyze mixed bacterial cultures that contained multiple
BWAs, e.g., B. anthracis mixed with B. thuringiensis kurstaki
and Y. pestis mixed with F. tularensis, in varying ratios.
We prepared 2 primer pools for the 7 BWAs of interest, and each pool
contained 1 primer pair specific for each BWA. Figure
2 shows
the amplification of BWAs in each mixed culture sample using primer pools
I and II. The amplified PCR products were subjected to multiplexed array
detection with each BWA represented by at least 2 probe types. The Appendix
Figure shows the results of simultaneous detection of BWAs in different
mixed culture samples after amplification with primer pool I (Appendix
Figure, panel A) and pool II (Appendix
Figure, panel B). For the mixtures of B. anthracis and B.
thuringiensis kurstaki, both probes BTK1 and BTK2 gave positive
signals, as did probes BA1, BA2, and BA4, which indicates the
presence of B.
anthracis and B. thuringiensis kurstaki. Since the primer
pair specific for B. anthracis in primer pool I and pool II corresponded
to the BA2 and BA4 sequences, respectively, no positive signals were
observed from the other BA probes (BA3, BA5, and BA6); no cross-reactions
were seen between them except for probes BA1 and BA2 (Appendix
Table 2 [93
KB, 1 page]). For mixtures of Y. pestis and F. tularensis,
differentiating 2 bands (Figure 2B, lane 9 and
lane 10) on the gel is difficult because the product size is similar;
however, positive signals from the respective probes after hybridization
showed these 2 BWAs in the mixed culture samples (Appendix
Figure, panel B). Array detection in conjunction with multiplex
PCR is advantageous in that it not only simultaneously identifies
target BWAs but also minimizes the possibility of misinterpreting
PCR results because it adds an additional level of specificity.
With gel analysis only, PCR results are usually complicated because
of nonspecific amplification during multiplex PCR with environmental
samples.
Since real environmental samples will likely involve complex matrices
with many potential interferents, the performance of the multiplexed array
was further assessed with wastewater spiked with individual autoclaved
bacterial cultures of BWAs at various volumetric dilution factors (1:3
and 1:10) (Appendix Table 3). Both
primer pools were applied to all spiked wastewater samples for multiplex
PCR. The probes on the multiplexed array gave positive responses only
to the amplified PCR products of interest, without responding to any nonspecifically
amplified products. Appendix Figure, panel
C gives an example of array detection of the amplified BWAs from spiked
wastewater samples (1:10 dilution) with primer pool I. BWAs seeded into
wastewater at various dilution factors were all identified successfully
within 30 minutes of hybridization.
In summary, this fiber-optic, microsphere-based array platform provides
fast, sensitive, and simultaneous identification of BWAs with high accuracy.
The high density of this array format can accommodate additional probe
types while still maintaining a high redundancy for each probe type on
the array. Additional probe types could be added to the array without
affecting the performance of the existing microspheres. The ability to
expand the probe types in the array opens up the opportunity to incorporate
a large number of potential BWAs when their genome sequences become available.
As a result, the multiplicity of arrays could be increased by incorporating
an even broader class of potential BWAs and other pathogens, leading to
a universal array for all pathogenic agents of interest.
Acknowledgments
We are grateful
to Illumina, Inc. for designing the probe sequences and primers and
the Naval Medical Research Command for providing the autoclaved cultures
of BWAs used in this study.
This work is funded
by the Office of Naval Research through a grant from the Technical Support
Working Group.
Ms Song is a graduate
student of chemistry at Tufts University. Her research interests include
applications of DNA microarrays and microarray-based detection of biological
warfare agents and other infectious biological agents.
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Table. Detection limits
of real samples determined with polymerase chain reaction followed
by array detection |
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|
Organism |
DNA copies/mL |
|
|
Bacillus anthracis |
103 |
|
B. thuringiensis kurstaki |
102 |
|
Vaccinia virus |
102 |
|
Yersinia pestis |
102 |
|
Francisella tularensis |
103 |
|
Clostridium botulinum |
103 |
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Suggested citation
for this article:
Song L, Ahn S, Walt
DR. Detecting biological warfare agents. Emerg Infect Dis [serial on the
Internet]. 2005 Oct [date cited]. Available from http://www.cdc.gov/ncidod/EID/vol11no10/05-0269.htm
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