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针对布鲁氏菌A细胞壁多糖抗原的单克隆Fab的分辨率为2.45埃的晶体结构。

Crystal structure to 2.45 A resolution of a monoclonal Fab specific for the Brucella A cell wall polysaccharide antigen.

作者信息

Rose D R, Przybylska M, To R J, Kayden C S, Oomen R P, Vorberg E, Young N M, Bundle D R

机构信息

Ontario Cancer Institute, University of Toronto, Canada.

出版信息

Protein Sci. 1993 Jul;2(7):1106-13. doi: 10.1002/pro.5560020705.

Abstract

The atomic structure of an antibody antigen-binding fragment (Fab) at 2.45 A resolution shows that polysaccharide antigen conformation and Fab structure dictated by combinatorial diversity and domain association are responsible for the fine specificity of the Brucella-specific antibody, YsT9.1. It discriminates the Brucella abortus A antigen from the nearly identical Brucella melitensis M antigen by forming a groove-type binding site, lined with tyrosine residues, that accommodates the rodlike A antigen but excludes the kinked structure of the M antigen, as envisioned by a model of the antigen built into the combining site. The variable-heavy (VH) and variable-light (VL) domains are derived from genes closely related to two used in previously solved structures, M603 and R19.9, respectively. These genes combine in YsT9.1 to form an antibody of totally different specificity. Comparison of this X-ray structure with a previously built model of the YsT9.1 combining site based on these homologies highlights the importance of VL:VH association as a determinant of specificity and suggests that small changes at the VL:VH interface, unanticipated in modeling, may cause significant modulation of binding-site properties.

摘要

分辨率为2.45埃的抗体抗原结合片段(Fab)的原子结构表明,由组合多样性和结构域缔合决定的多糖抗原构象和Fab结构是布鲁氏菌特异性抗体YsT9.1精细特异性的原因。它通过形成一个由酪氨酸残基排列的凹槽型结合位点,将流产布鲁氏菌A抗原与几乎相同的羊种布鲁氏菌M抗原区分开来,该结合位点容纳棒状A抗原,但排除了M抗原的扭结结构,正如结合位点中构建的抗原模型所设想的那样。重链可变区(VH)和轻链可变区(VL)分别源自与先前解析结构中使用的两个基因密切相关的基因,即M603和R19.9。这些基因在YsT9.1中组合形成具有完全不同特异性的抗体。将此X射线结构与基于这些同源性先前构建的YsT9.1结合位点模型进行比较,突出了VL:VH缔合作为特异性决定因素的重要性,并表明在建模中未预料到的VL:VH界面处的微小变化可能会导致结合位点性质的显著调节。

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