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利用与蛋白A片段融合的Fv片段开发具有多价性的人工抗体系统。

Development of an artificial antibody system with multiple valency using an Fv fragment fused to a fragment of protein A.

作者信息

Ito W, Kurosawa Y

机构信息

Institute for Comprehensive Medical Science, Fujita Health University, Aichi, Japan.

出版信息

J Biol Chem. 1993 Sep 25;268(27):20668-75.

PMID:8376416
Abstract

In antigen-antibody interactions, the high avidity of antibodies for their specific antigens can be achieved both by exploiting the high affinity of each binding site and by multivalence of antibodies. In this study, we developed artificial antibodies with multiple valency. The Fv fragments of an antibody fused with one and with two domains of the Fc-binding protein A from Staphylococcus aureus (designated Fv-P and Fv-PP, respectively) were expressed in secreted forms in Escherichia coli. Their physical characteristics were examined. The Fv portions of Fv-P and Fv-PP had virtually the same affinity for the antigen as that of the original Fv molecules, and each protein A-derived domain could be bound to IgG. When Fv-P was mixed with IgG, the complex formed was composed of two Fv-P molecules and one IgG molecule. In the case of Fv-PP, a complex composed of three Fv-PP molecules and two IgG molecules was preferentially formed. Analysis of surface plasmon resonance in a BIAcore system indicated multivalency of these complexes for antigens. There was 3.5-fold decrease in the dissociation constant of the complex between Fv-PP and the antigen upon the addition of IgG. The use of these complexes as reagents in enzyme-linked immunosorbent assay and Western blotting gave much stronger signals than Fv, Fv-P, and Fv-PP alone.

摘要

在抗原-抗体相互作用中,抗体对其特异性抗原的高亲和力既可以通过利用每个结合位点的高亲和力来实现,也可以通过抗体的多价性来实现。在本研究中,我们开发了具有多价性的人工抗体。将与来自金黄色葡萄球菌的Fc结合蛋白A的一个和两个结构域融合的抗体的Fv片段(分别命名为Fv-P和Fv-PP)以分泌形式在大肠杆菌中表达。检测了它们的物理特性。Fv-P和Fv-PP的Fv部分对抗原的亲和力与原始Fv分子几乎相同,并且每个源自蛋白A的结构域都可以与IgG结合。当Fv-P与IgG混合时,形成的复合物由两个Fv-P分子和一个IgG分子组成。在Fv-PP的情况下,优先形成由三个Fv-PP分子和两个IgG分子组成的复合物。在BIAcore系统中对表面等离子体共振的分析表明这些复合物对抗原具有多价性。加入IgG后,Fv-PP与抗原之间复合物的解离常数降低了3.5倍。在酶联免疫吸附测定和蛋白质印迹中使用这些复合物作为试剂比单独使用Fv、Fv-P和Fv-PP产生的信号要强得多。

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