Serum samples were analysed for the presence of (a) IgG against VP1+VP2 using recombinant native conformational antigens by ELISA test (b) IgG against VP2 using recombinant native conformational antigens by ELISA test and (c) IgG against VP1 and against VP2 using denatured linear antigens by Western blot. Out of the 446 samples examined, 353 were positive for specific B19 IgG and out of these, 98.6 % proved positive in the ELISA assay using conformational VP1+VP2 antigens, 94.6% proved positive in the ELISA assay using conformational VP2 antigens, 89.5% were positive at the Western blot assay using denatured linear VP1 and VP2 antigens, with all proving positive for linear VP1 and only 29.5% out of the positive samples proving positive for linear VP2. Since all samples positive by Western blot proved positive by ELISA, our data show that recombinant capsids obtained either with VP1+VP2 or with VP2 alone, used in ELISA, are very useful for detecting the immune response against both conformational and native linear epitopes of B19 structural proteins although some sera may have antibodies directed exclusively against VP1+VP2 antigens and few may have antibodies directed exclusively against VP2 antigens alone.

Manaresi E, Gallinella G., Venturoli S., Zerbini M., Musiani M. (2004). Detection of parvovirus B19 IgG: choice of antigens and serological tests. JOURNAL OF CLINICAL VIROLOGY, 29, 51-53 [10.1016/S1386-6532(03)00088-X].

Detection of parvovirus B19 IgG: choice of antigens and serological tests

MANARESI, ELISABETTA;GALLINELLA, GIORGIO;VENTUROLI, SIMONA;ZERBINI, MARIALUISA;MUSIANI, MONICA
2004

Abstract

Serum samples were analysed for the presence of (a) IgG against VP1+VP2 using recombinant native conformational antigens by ELISA test (b) IgG against VP2 using recombinant native conformational antigens by ELISA test and (c) IgG against VP1 and against VP2 using denatured linear antigens by Western blot. Out of the 446 samples examined, 353 were positive for specific B19 IgG and out of these, 98.6 % proved positive in the ELISA assay using conformational VP1+VP2 antigens, 94.6% proved positive in the ELISA assay using conformational VP2 antigens, 89.5% were positive at the Western blot assay using denatured linear VP1 and VP2 antigens, with all proving positive for linear VP1 and only 29.5% out of the positive samples proving positive for linear VP2. Since all samples positive by Western blot proved positive by ELISA, our data show that recombinant capsids obtained either with VP1+VP2 or with VP2 alone, used in ELISA, are very useful for detecting the immune response against both conformational and native linear epitopes of B19 structural proteins although some sera may have antibodies directed exclusively against VP1+VP2 antigens and few may have antibodies directed exclusively against VP2 antigens alone.
2004
Manaresi E, Gallinella G., Venturoli S., Zerbini M., Musiani M. (2004). Detection of parvovirus B19 IgG: choice of antigens and serological tests. JOURNAL OF CLINICAL VIROLOGY, 29, 51-53 [10.1016/S1386-6532(03)00088-X].
Manaresi E; Gallinella G.; Venturoli S.; Zerbini M.; Musiani M.;
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11585/4901
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