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Serological Response in RT-PCR Confirmed H1N1-2009 Influenza A by Hemagglutination Inhibition and Virus Neutralization Assays: An Observational Study

Authors :
Brown, J
Chen, MI
Barr, IG
Koh, GCH
Lee, VJ
Lee, CPS
Shaw, R
Lin, C
Yap, J
Cook, AR
Tan, BH
Loh, JP
Barkham, T
Chow, VTK
Lin, RTP
Leo, Y-S
Brown, J
Chen, MI
Barr, IG
Koh, GCH
Lee, VJ
Lee, CPS
Shaw, R
Lin, C
Yap, J
Cook, AR
Tan, BH
Loh, JP
Barkham, T
Chow, VTK
Lin, RTP
Leo, Y-S
Publication Year :
2010

Abstract

BACKGROUND: We describe the serological response following H1N1-2009 influenza A infections confirmed by reverse-transcriptase polymerase chain reaction (RT-PCR). METHODOLOGY AND PRINCIPAL FINDINGS: The study included patients admitted to hospital, subjects of a seroepidemiologic cohort study, and participants identified from outbreak studies in Singapore. Baseline (first available blood sample) and follow-up blood samples were analyzed for antibody titers to H1N1-2009 and recently circulating seasonal influenza A virus strains by hemagglutination inhibition (HI) and virus micro-neutralization (VM) assays. 267 samples from 118 cases of H1N1-2009 were analyzed. Geometric mean titers by HI peaked at 123 (95% confidence interval, CI 43-356) between days 30 to 39. The chance of observing seroconversion (four-fold or greater increase of antibodies) was maximized when restricting analysis to 45 participants with baseline sera collected within 5 days of onset and follow-up sera collected 15 or more days after onset; for these participants, 82% and 89% seroconverted to A/California/7/2009 H1N1 by HI and VM respectively. A four-fold or greater increase in cross-reactive antibody titers to seasonal A/Brisbane/59/2007 H1N1, A/Brisbane/10/2007 H3N2 and A/Wisconsin/15/2009 H3N2 occurred in 20%, 18% and 16% of participants respectively. CONCLUSIONS AND SIGNIFICANCE: Appropriately timed paired serology detects 80-90% RT-PCR confirmed H1N1-2009; Antibodies from infection with H1N1-2009 cross-reacted with seasonal influenza viruses.

Details

Database :
OAIster
Publication Type :
Electronic Resource
Accession number :
edsoai.on1315694003
Document Type :
Electronic Resource