单克隆抗体多特异性的合成组合文库解析。

Peptide research Pub Date : 1995-09-01
C Pinilla, S Chendra, J R Appel, R A Houghten
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摘要

利用可溶性合成组合文库(SCL)系统地检测了一种抗多肽单克隆抗体的潜在多特异性。该SCL由400种不同的六肽混合物组成,每个混合物由超过130,000个肽组成,总计5000万个单个序列,浓度约为等摩尔。通过竞争性酶联免疫吸附试验(ELISA)筛选了400个组成该SCL的多肽混合物,以确定其抑制单克隆抗体与原免疫肽结合的能力。通过反复筛选和选择过程,从肽库的三种不同的肽混合物中获得单个肽。除了鉴定出该单克隆抗体识别的六残基抗原决定序列外,还发现另外两个六肽的结合亲和力比原始抗原决定序列高5- 10倍。这些肽序列表示类似物,其中原始抗原决定因素中的极性氨基酸(苏氨酸)被一个大的芳香氨基酸(色氨酸或酪氨酸)取代。抗原决定因子的肽类似物,从单个到多个取代,以及与免疫肽完全无关的肽序列,也被发现具有与原始免疫原相当的结合亲和力。目前的研究说明了scl在确定抗原抗体相互作用的替代结合基序方面的能力。以这种方式使用scl可能有助于阐明在抗原-抗体相互作用中发现的交叉反应性,多特异性和分子模仿的程度。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Elucidation of monoclonal antibody polyspecificity using a synthetic combinatorial library.

The potential polyspecificity of an antipeptide monoclonal antibody was systematically examined using a soluble synthetic combinatorial library (SCL). This SCL was composed of 400 different hexapeptide mixtures, each of which consisted of more than 130,000 peptides totalling 50 million individual sequences in approximately equimolar concentration. The 400 peptide mixtures making up this SCL were screened by competitive enzyme-linked immunosorbent assay (ELISA) for their ability to inhibit monoclonal antibody binding to the original immunizing peptide. Individual peptides were derived from three different peptide mixtures of the peptide library through an iterative screening and selection process. In addition to the identification of the six-residue antigenic determinant recognized by this monoclonal antibody, two other hexapeptides were found to have binding affinities 5- to 10-fold higher than the original antigenic determinant sequence. These peptide sequences represent analogs in which a polar amino acid (threonine) in the original antigenic determinant was substituted with a large, aromatic amino acid (either tryptophan or tyrosine). Peptide analogs of the antigenic determinant, ranging from single to multiple substitutions, as well as peptide sequences completely unrelated to the immunizing peptide, were also identified having binding affinities comparable to the original immunogen. The present study illustrates the power of SCLs for the determination of alternative binding motifs for antigen antibody interactions. The use of SCLs in this manner may help to elucidate the extent of cross-reactivity, polyspecificity and molecular mimicry found in antigen-antibody interactions.

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