犬细小病毒
衣壳
生物
细小病毒
病毒学
表位
病毒
单克隆抗体
小鼠微小病毒
抗原
抗原变异
水貂
细小病毒科
分子生物学
抗体
遗传学
生态学
作者
M. Lisa Strassheim,A. Gruenberg,P. Veijalainen,Jean-Yves Sgro,Colin R. Parrish
出处
期刊:Virology
[Elsevier BV]
日期:1994-01-01
卷期号:198 (1): 175-184
被引量:177
标识
DOI:10.1006/viro.1994.1020
摘要
The 25-nm diameter parvovirus capsid is assembled from 60 copies of a sequence common to the overlapping VP1 and VP2 proteins. Here we examine the epitope specificity's of 28 monoclonal antibodies (MAb) prepared against canine parvovirus (CPV), feline panleukopenia virus (FPV), and raccoon-dog parvovirus or blue (Arctic) fox parvovirus. Comparing the reactivity of those MAb with various MAb-selected escape mutants, or with natural variants of CPV or mink enteritis virus (MEV) which differ at known sequences, showed that the binding of 20 of those MAb was strongly affected by variations of two regions on the threefold spike of the CPV capsid. One region was adjacent to the tip of the threefold spike, and the second was around VP2 residue 300, on the shoulder of that structure. MAb recognizing both antigenic sites efficiently neutralized the virus infectivity and inhibited hemagglutination. Mutations leading to natural antigenic variation have also been observed in both those sites in naturally variant strains of CPV or MEV, suggesting that they are important antigenic structures on these parvoviruses. The bindings of several MAb were not affected by the mutations at those antigenic sites, indicating that they recognized other, and perhaps conserved, structures.
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