ISSN: 1080-6059
Theo P. Sloots,*††‡§1 Ian M. Mackay,*†‡1 Seweryn Bialasiewicz,*† Kevin C. Jacob,*†‡ Emily
McQueen,*† Gerald B. Harnett,¶ David J. Siebert,§ I. Brent Masters,* Paul R.
Young,‡ and Michael D. Nissen*†‡§
*Royal Children's Hospital and Health Service District, Brisbane, Queensland, Australia;
†Clinical Medical Virology Centre at University of Queensland, Brisbane, Queensland, Australia; ‡University
of Queensland, Brisbane, Queensland, Australia; §Queensland Health Pathology
Service, Brisbane, Queensland, Australia; and ¶PathWest Laboratory Medicine,
Perth, Western Australia, Australia
Suggested citation for this article
We examined 10,025 respiratory samples collected for 4 years (2001–2004) and found a 7.1% average annual incidence of human metapneumovirus. The epidemic peak of infection was late winter to spring, and genotyping showed a change in predominant viral genotype in 3 of the 4 years.
Human metapneumovirus (HMPV) is now recognized as a substantial cause of acute respiratory infection, particularly in children; it has phenotypic and clinical characteristics that are similar to those of respiratory syncytial virus (RSV) (1,2). HMPV is ubiquitous; it infects most children at an early age, and distinct epidemic peaks are reported in the winter months (1,3–6). However, many of theses studies were conducted in the Northern Hemisphere and involved samples collected during a relatively short period; few data exist from extended studies over several years that involve populations in other parts of the world.
Although 2 main HMPV types are recognized (A and B) (1,3,7), each with 2 subtypes (A1, A2; B1, B2) (8), the extent of genetic variation of circulating HMPV subtypes over time has not been extensively examined. We sought to determine the incidence and seasonal distribution of HMPV in an Australian population from 2001 to 2004 and to establish the pattern of genotype distribution during those 4 years by examining the genetic variability of the P gene in 640 of 707 HMPV-positive samples.
The necessary ethics approval for this study was obtained from the Royal Children's Hospital ethics committee. We collected nasopharyngeal aspirate (NPA) specimens from January 2001 through December 2004 from patients with acute lower respiratory tract infection in Queensland, Australia. Patients were from 3 months to 93 years of age (mean 8.2 years, median 1.37 years), and 78.1% of specimens were from children <5 years of age. Nucleic acids were extracted from 0.2 mL of each NPA specimen by using the High Pure Viral Nucleic Acid kit (Roche Diagnostics, Mannheim, Germany), according to the manufacturer's instructions. Extracts were analyzed for HMPV sequences by reverse transcriptase PCR (9). For samples collected during 2001 and 2002, other viral respiratory pathogens were detected by using a direct fluorescent antibody assay (DFA) in combination with a culture-augmented DFA method (10). For samples collected in 2003 and 2004, these pathogens were detected by multiplex PCR (10).
Of 10,025 NPA specimens tested, 707 were positive for HMPV, for an overall incidence of 7.1% during the 4 years. The youngest HMPV-positive patient was 4 months old, and the oldest was 79 years. In children (<18 years of age) the incidence of virus was 7.4%, and 91.9% of HMPV-positive children were <5 years of age. The seasonal distribution of HMPV infection showed a distinctive pattern for each of the 4 years studied (Figure 1). In 2001, HMPV showed broad seasonal activity; incidence was >5% in 3 consecutive seasons (autumn, winter, and spring) and peaked at 10.6% in the spring (September–November). In 2002 and 2004, most HMPV activity was in spring, (incidence of 13.6% and 15.4%, respectively), with little evidence during autumn (March–May). In 2003, the peak incidence of 9.0% occurred in winter (June–August) and persisted into spring (5.4%). In all years, virus was present well into summer (December–February), with an incidence ranging from 2.5% to 5.2%. On examination of those samples collected in 2003 and 2004, which were all previously analyzed for common respiratory viruses by PCR, HMPV was the most frequently detected respiratory virus in children during the spring of each year. Expressed as an annual average over the 4 years studied, the predominant viral pathogen was RSV (9.2%), followed by HMPV (7.1%), influenza A (3.5%), parainfluenza virus 3 (2.3%), and adenovirus (1.3%). In 6.8% of HMPV-positive cases, evidence of co-infection with another respiratory virus was seen; 20 patients were concurrently infected with an adenovirus, 10 with influenza A virus, 8 with RSV, 9 with parainfluenza virus 3, and 1 with parainfluenza virus 2.
Amplification products generated directly from 640 HMPV-positive NPA specimens were genotyped as previously described (11) (GenBank accession nos. DQ112292–DQ112320 and DQ121378–DQ121384). Data showed that all 4 viral subtypes cocirculated during each of the 4 years studied (Table 1, Figure 2). However, a different subtype predominated during 3 of the 4 years: HMPV subtype A1 was dominant in 2001, subtype A2 in 2002 and 2003, and subtype B1 in 2004 (Table 1).
Clinical records from 273 patients who were positive for HMPV were scrutinized, and data describing clinical features and length of hospital stay were recorded. Of these patients, 203 (74.4%) were admitted to hospital with a median length of admission of 3 days and a mean of 6.5 days. The predominant clinical features were cough (63%), rhinorrhea (61%), respiratory crackles/crepitations (60%), and fever (57%) (Table 2). Ninety (33.9%) of the 273 patients had a chest radiograph, and 77 (85.6%) patients showed bilateral parahilar peribronchial infiltrates consistent with a lower respiratory tract infection. Disease severity of the 273 HMPV-positive patients was classified as mild (46.8%), moderate (42.5%), and severe (10.7%), based on the use of supplemental oxygen and fluids and length of hospital stay.
This study of HMPV infection is the largest so far reported. The results of recent, similar studies suggested that peak periods of infection with HMPV predominate during winter in the Northern Hemisphere. However, this finding has not been extensively examined over an extended period with a large, continuous sample. Our study found that the peak period of HMPV infection in Queensland, Australia, occurs predominantly in spring (August–October) but that HMPV can be detected in every month. This finding suggests that HMPV activity, like RSV activity, occurs in the community throughout the year, and peaks of infection are a result of seasonal environmental factors.
Although RSV predominated in all years, HMPV was the second most frequently detected virus in each year studied. The low rate of co-infection of HMPV with other respiratory viruses (including RSV) suggests that co-infection may not be common in our community. When analyzing disease severity in this sample with a 2-sided test of proportions, we saw no significant difference between patients with a co-infection and those without. Therefore, our data did not support the suggestion by others that co-infection of HMPV with RSV or other viral respiratory pathogens is a risk factor for severe disease (6).
The shift in predominant HMPV genotype observed in this study was similar to those reported for RSV and influenza viruses (6) and can be attributed to changes in immunity of the population in response to antigenic differences between the predominant circulating strains (12,13). However, a relationship between genotype and disease severity, as previously established for RSV (14,15), did not appear to apply for HMPV, but we plan to examine this relationship further.
The clinical features associated with HMPV infection in this study were not sufficiently distinctive to clinically differentiate it from other respiratory viral infections in children, particularly those attributed to RSV. In addition, few patients (10.6%) had severe disease, but most (76%) were sufficiently ill to be admitted and treated in the hospital for >3 days, which represents a substantial amount in healthcare costs.
Finally, this comprehensive study, conducted for 48 months, is the first one aimed at establishing an accurate estimate of the incidence and seasonal distribution of HMPV infection and to determine the genetic variation of HMPV circulating in our population. The clinical spectrum of infection in a substantial proportion of HMPV-positive patients has been described, and studies are continuing to fully elucidate the clinical effect of infection with this virus in our community.
We thank the staff of the Microbiology Division of the Queensland Health Pathology Service, Royal Brisbane and Women's Hospital. We also acknowledge the Directors of Paediatrics, Queensland Health, who gave permission to review the medical records of HMPV-positive patients.
This study was supported by the Royal Children's Hospital Foundation grants I 922-034 and R 912-009, the Woolworths Fresh Futures Appeal, and the National Health and Medical Research Council, Australia, project grant 243702.
Dr Sloots is the director of the research section of the Queensland Paediatric Infectious Diseases Laboratory at Sir Albert Sakzewski Virus Research Centre. His main research interests are in pediatric infectious diseases, particularly viral respiratory disease.
Figure 1. Seasonal incidence of human metapneumovirus, Queensland, Australia, 2001–2004...
Figure 2. Phylogenetic
analysis of the 182-nucleotide fragment of the phosphoprotein gene fragment of human
metapneumovirus detected in respiratory samples collected in Australia...
Table 1. Distribution of human metapneumovirus (HMPV) subtypes in Queensland, Australia, 2001–2004
Table 2. Signs and
symptoms noted with human metapneumovirus infection (N = 273)
Sloots TP, Mackay IM, Bialasiewicz S, Jacob KC, McQueen E, Harnett GB, et al. Human metapneumovirus, Australia, 2001–2004. Emerg Infect Dis [serial on the Internet]. 2006 Aug [date cited]. Available from http://www.cdc.gov/ncidod/EID/vol12no08/05-1239.htm
1These authors contributed equally to this study.
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Theo P. Sloots, Queensland Pediatric Infectious Diseases Laboratory, Sir Albert Sakzewski Virus Research Centre, Royal Childrens Hospital and Health Service District, Herston Rd, Herston, Queensland, Australia 4029; email: t.sloots@uq.edu.au
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