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基于多克隆抗体的亲和捕获生成单特异性抗体。

Generation of monospecific antibodies based on affinity capture of polyclonal antibodies.

机构信息

Department of Biotechnology, AlbaNova University Center, Royal Institute of Technology, 10691 Stockholm, Sweden.

出版信息

Protein Sci. 2011 Nov;20(11):1824-35. doi: 10.1002/pro.716. Epub 2011 Oct 12.

Abstract

A method is described to generate and validate antibodies based on mapping the linear epitopes of a polyclonal antibody followed by sequential epitope-specific capture using synthetic peptides. Polyclonal antibodies directed towards four proteins RBM3, SATB2, ANLN, and CNDP1, potentially involved in human cancers, were selected and antibodies to several non-overlapping epitopes were generated and subsequently validated by Western blot, immunohistochemistry, and immunofluorescence. For all four proteins, a dramatic difference in functionality could be observed for these monospecific antibodies directed to the different epitopes. In each case, at least one antibody was obtained with full functionality across all applications, while other epitope-specific fractions showed no or little functionality. These results present a path forward to use the mapped binding sites of polyclonal antibodies to generate epitope-specific antibodies, providing an attractive approach for large-scale efforts to characterize the human proteome by antibodies.

摘要

描述了一种基于定位多克隆抗体线性表位并使用合成肽进行连续表位特异性捕获来生成和验证抗体的方法。选择了针对四个可能涉及人类癌症的蛋白质(RBM3、SATB2、ANLN 和 CNDP1)的多克隆抗体,并生成了针对多个非重叠表位的抗体,随后通过 Western blot、免疫组织化学和免疫荧光进行了验证。对于这四种蛋白质,针对不同表位的单特异性抗体在功能上存在显著差异。在每种情况下,至少获得了一种具有所有应用程序全功能的抗体,而其他表位特异性部分则没有或几乎没有功能。这些结果为利用多克隆抗体的结合位点生成表位特异性抗体提供了一条前进的道路,为通过抗体大规模努力描绘人类蛋白质组提供了一种有吸引力的方法。

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