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首页> 外文期刊>Journal of Virology >Anti-idiotypic antibodies to a polyomavirus monoclonal antibody recognize cell surface components of mouse kidney cells and prevent polyomavirus infection.
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Anti-idiotypic antibodies to a polyomavirus monoclonal antibody recognize cell surface components of mouse kidney cells and prevent polyomavirus infection.

机译:抗独特型抗体的抗体抗体识别小鼠肾细胞的细胞表面成分,并预防多瘤病毒感染。

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摘要

Anti-idiotypic antibodies have been successfully used to identify and isolate the receptor for several cell ligands. To prepare an immunologic probe for identification of the polyomavirus receptor on mouse kidney cells, polyclonal antisera against antipolyomavirus antibodies were prepared in rabbits. Fab fragments of the previously characterized monoclonal antibody E7, which neutralizes polyomavirus infection, were used for immunization (S. J. Marriott and R. A. Consigli, J. Virol. 56:365-372, 1985). Sera containing the greatest anti-idiotype activity were identified by enzyme-linked immunosorbent assay (ELISA) and purified by a series of affinity columns. The anti-idiotypic antibodies recognized the E7 idiotope in an ELISA, and anti-idiotype binding could be inhibited by preincubation of E7 monoclonal antibody with polyomavirus virions. When mixed with anti-idiotype immunoglobulin G (IgG), E7 was no longer capable of binding or immunoprecipitating polyomavirus virions or neutralizing polyomavirus infection. Direct immunofluorescence showed anti-idiotype IgG reactivity with a cell surface component of mouse kidney cells. Anti-idiotype F(ab')2 effectively competed with polyomavirus for binding to mouse kidney cells and displayed binding kinetics similar to those of polyomavirus. Virus infection of mouse kidney cells was blocked in a dose-dependent manner following treatment of the cells with anti-idiotype IgG. The anti-idiotype identified several proteins (95, 50, and 24 to 31 kilodaltons) in an immunoblot of mouse kidney cell membrane proteins but reacted predominantly with a single 50-kilodalton protein in a radioimmunoassay. The anti-idiotype failed to react with virus proteins in three assays, including ELISA, immunoprecipitation, and immunoblotting. The implications of this work for future identification and characterization of the polyomavirus receptor on mouse kidney cells are discussed.
机译:已经成功地用于鉴定和分离几种细胞配体的受体的抗肌型抗体。为了制备免疫探针,用于鉴定小鼠肾细胞上的多瘤受体,在兔中制备针对抗抗抗oloMavirus抗体的多克隆抗血清。将先前表征的单克隆抗体E7的Fab片段中和多瘤感染,用于免疫(S.J.Marriott and R. A. Consgli,J.Virol。56:365-372,1985)。通过酶联免疫吸附测定(ELISA)鉴定含有最大抗独特型活性的血清,并通过一系列亲和柱纯化。抗独特型抗体在ELISA中识别E7恋物癖,并且可以通过用聚瘤病毒粒子的E7单克隆抗体预孵育来抑制抗独立型结合。当与抗独特型免疫球蛋白G(IgG)混合时,E7不再能够结合或免疫沉淀多马病毒病毒病毒藻或中和多马力病毒感染。直接免疫荧光显示抗独立型IgG反应性与小鼠肾细胞的细胞表面成分。抗独立型F(AB')2有效地竞争PolyomaVirus,用于与小鼠肾细胞结合并显示与多聚瘤毒脉相似的结合动力学。用抗独立型IgG处理细胞,以剂量依赖性方式阻断小鼠肾细胞病毒感染。抗独特型在小鼠肾细胞膜蛋白的免疫印迹中鉴定了几种蛋白质(95,50和24至31千杆杆罗罗氏蛋白,但在放射免疫测定中主要在单个50千倍珠蛋白中反应。抗独特型未能在三种测定中与病毒蛋白质反应,包括ELISA,免疫沉淀和免疫印迹。讨论了这项工作的含义,用于对小鼠肾细胞上的多容阀受体的未来鉴定和表征。

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