A subtype-specific peptide-based enzyme immunoassay for detection of antibodies to the G protein of human respiratory syncytial virus is more sensitive than routine serological tests

J.P.M. Langedijk, A.H. Brandenburg, W.G.J. Middel, A.B. Osterhaus, R.H. Meloen, J.T. van Oirschot

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    Abstract

    Peptides deduced from the central conserved region (residues 158 to 189) of protein G of human respiratory syncytial virus (HRSV) subtypes A and B were used as antigens in subtype-specific enzyme-linked -bent assays (G- peptide ELISAs). These G-peptide ELlSAs were compared with seven other serological assays to detect HRSV infection: ELlSAs based on complete protein G, on fusion protein F, and on nucleoprotein N; a complement fixation assay; a virus neutralization test; and ELISAs for the detection of immunoglobulin A (IgA) or IgM antibodies specific for HRSV. In paired serum samples from patients with HRSV infection, more infections were diagnosed by the G- peptide ELISA (67%) than by all other serological tests combined (48%). Furthermore, for 16 of 18 patients (89%), the G-peptide ELISAs were able to differentiate between antibodies against HRSV subtypes A and B. This study shows that peptides corresponding to the central conserved region of the attachment protein G of HRSV can successfully be used as antigens in immunoassays. The G-peptide ELISA appeared to be more sensitive than conventional tests for the detection of HRSV antibody titer rises.
    Original languageEnglish
    Pages (from-to)1656-1660
    JournalJournal of Clinical Microbiology
    Volume35
    Issue number7
    Publication statusPublished - 1997

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