禽白血病毒单克隆抗体的特性
CHARACTERIZATION OF MONOCLONAL ANTIBODIES TO AVIAN LEUKOSIS VIRUSES
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摘要: 建立了分泌抗禽白血病毒(ALV)结构蛋白P27和P19的单克隆抗体(McAb)杂交瘤细胞。酶联免疫吸附试验(ELISA),McAb-6AL20(属于IgG1)分别与外源性ALV:A.B.D亚群的RPL-40、AMV、RAV-2和Carr-Zilber RSV(CZ-RSV)发生特异性反应,而不与内源性ALV:RAV-O(E亚群)发生反应。McAb-6AL22(属于IgG1)除了上述特性外,还能与劳斯氏肉瘤病毒Prague株(Prc-RSV、属于C亚群)发生反应。这二个McAb均能与〔35S〕甲硫氨酸标记的RPL-40和RAV-1病毒的P19蛋白出现免疫沉淀。但是,它们不与RAV-O病毒的P19蛋白发生免疫沉淀。所以,McAb可用于区别ALV结构蛋白P19(亚群特异性位点的多肽)。应用这二个McAb进行ELISA和免疫沉淀与聚丙烯酰胺凝胶电泳试验可区分RPL-40和RAV-O感染。McAb-6AL42(属于IgG2a)可与以上几个亚群(A.B.C和D)的毒株发生反应,其ELISA的抗体滴度比与RAV-O(E亚群)毒株高1000倍以上。McAb-6AL42可与P27和pr76(群特异性抗原的前体蛋白)发生免疫沉淀。试验用McAb-6AL42作为第一抗体和兔抗P27血清的过氧化物酶标记物作为第二抗体(指示抗体)建立了双抗体夹心ELISA试验。用这种ELISA试验可区分未经稀释的卵蛋白中RAV-O和RPL-40群特异性抗原。Abstract: Hybridoma cell lines secreting monoclonal antibody (MCA) to avian leukosis virus (ALV) structural proteins p27 and p19 have been established. MCA 6AL20 (IgG1 isotype) reacted with RPL-40, AMV, RAV-2 and Carr-Zilber RSV (CZ-RSV).representing exogenous ALV subgroups A, B and D, respectively, but not the endogenous virus RAV-0 (subgroup E) in an indirect enzyme-linked immunosorbent assay (ELISA). MCA 6AL22 reacted as above and, in addition, reacted with the Prague strain of Rous sarcoma virus (PrC-RSV), subgroup C. Both MCAs im-munoprecipitated p19 from 35S-methionine-labeled RPL-40 or RAV-1,but not RAV-O infected chi-cken embryo fibroblasts (CEF). They can be used to differentiate exogenous from endogenous (RAV-O) infection either in an indirect antibody ELISA or by immunoprecipitation. A third MCA, 6AL42 (IgG2a isotype), reacted with exogenous viruses at an antibody titer up to 1,000-fold higher than with endogenous subgroup E, RAV-O virus in indirect ELISAs. MCA 6AL42 immunoprecipitated p27 and the group-specific antigen precursor protein, pr76, from cells infected with RPL-40, RAV-1 or RAV-O. A double antibody sandwich ELISA, using 6AL42 as the primary binding antibody and conjugated rabbit anti-p27 as the reporter antibody, differentiated between endogenous RAV-O and exogenous p27 antigen in undiluted albumen samples.
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[7] Crittenden, L, B.,xue E, J.Smith, 1984, A comparison of test materials for differentiaLiag avian leak osis virus group-specific antigens of exogenous and endogenous origin, Avian Dis, 28:1055 [8] De Boer, G. F. and A. D. E. Osterhaus. 1985, Application of moaoclonal antibodies in the avian leukosis virus gs antigen EL1SA。A vian Pathol. 14:3-55 [13] lgnjatovic, J., and T. J. Bagust. 1983. Practical application of ELISA for detection of vertical transmission of leukosis virus in commercial layer hens, Avian pathol, 12:515-519 [17] Parsons, S. J.,L. D. Wilson, C. M. Ely, J. T. Parsons, and D. C. Benjamin 1984, Monoclonal antibodies specific for the virion polypeptide, p27. of avian retrov:ruses, Hybridoma 3:25-31 [18] purchase, H. G.,and L. N. Payne, 1984, Leuhosis/sarcuma group, in:Diseases of Poultry, 8th Ed,(M. S. Hofstad. H. J. Barnes. B. W. Calnelt, W, M, Reid, and H. W. Yoder, eds.), pp. 360-405.Iowa State University Press, Ames, Iowa [20] Robinson, H. L., and R. N. Eisenman, 1934. New findings on the congenita; transmission of avian leukosis virus, Science 325:417-419 [21] Silva, R. F., and L. F. Lee, 1934, Monoclonal antibody-mediated immunoprecipitation of proteins from cells infected with Marek’s disease virus or turkey herpesvirus, Virology, 136:307-320. [25] Wilson,M. B. and P.K. Nakane, 1978. Recent developments in the periodate method of conjugating horseradish peroxidase (HRPO) to antibodies. In:Immunofluorescenee and Related Techniques (W. Knapp, K. Holubar, and G. Wicks, eds.)pp, 215-234. Elsevier/Nurth Holland Biomedical Press, Amsterriam, Holland
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