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作为与大肠杆菌鞭毛蛋白融合体的黏附肽的功能表达。

Functional expression of adhesive peptides as fusions to Escherichia coli flagellin.

作者信息

Westerlund-Wikström B, Tanskanen J, Virkola R, Hacker J, Lindberg M, Skurnik M, Korhonen T K

机构信息

Department of Biosciences, University of Helsinki, Finland.

出版信息

Protein Eng. 1997 Nov;10(11):1319-26. doi: 10.1093/protein/10.11.1319.

DOI:10.1093/protein/10.11.1319
PMID:9514121
Abstract

An expression system for studying epitopes of adhesion proteins based on fusion of gene fragments into fliC(H7) of Escherichia coli is described. We constructed the system by an in-frame insertion of DNA fragments encoding one, two or three of the fibronectin-binding D repeats present in the fibronectin-binding protein A (FnBPA) of Staphylococcus aureus, into the fliC(H7) gene region encoding the variable domain of the H7 flagellin. The constructs were expressed by in trans complementation in the E. coli strain JT1 which harbours knock-out mutations for the expression of FliC as well as of the mannoside-binding fimbrial adhesin. The resulting chimeric flagella, which contained 39, 77 or 115 heterologous amino acid residues, efficiently bound soluble and immobilized human plasma and cellular fibronectin, and the binding was most efficient with the flagella containing the three D repeats of FnBPA. The chimeric flagella bound to frozen sections of human kidney and to cultured human cells. Antibodies raised against the chimeric flagella bound to Protein A-deficient S. aureus cells and inhibited the binding of staphylococci to immobilized fibronectin. We also expressed peptides, ranging in size between 48 and 302 amino acids, of the collagen-binding YadA adhesin of Yersinia enterocolitica. A fragment of 302 amino acids representing the middle region of YadA was needed for collagen binding. Chimeric flagellar filaments expressing hundreds of intimately associated adhesive epitopes offer versatile tools to analyze adhesin-receptor interactions and functional epitopes of adhesion proteins.

摘要

描述了一种基于将基因片段融合到大肠杆菌fliC(H7)中来研究粘附蛋白表位的表达系统。我们通过将编码金黄色葡萄球菌纤维连接蛋白结合蛋白A(FnBPA)中一个、两个或三个纤维连接蛋白结合D重复序列的DNA片段读框内插入到编码H7鞭毛蛋白可变结构域的fliC(H7)基因区域,构建了该系统。构建体通过在大肠杆菌菌株JT1中的反式互补表达,该菌株对FliC以及甘露糖苷结合菌毛粘附素的表达具有敲除突变。产生的嵌合鞭毛含有39、77或115个异源氨基酸残基,能有效结合可溶性和固定化的人血浆及细胞纤维连接蛋白,且对于含有FnBPA三个D重复序列的鞭毛,结合效率最高。嵌合鞭毛与人肾冷冻切片及培养的人细胞结合。针对嵌合鞭毛产生的抗体与缺乏蛋白A的金黄色葡萄球菌细胞结合,并抑制葡萄球菌与固定化纤维连接蛋白的结合。我们还表达了小肠结肠炎耶尔森菌胶原结合YadA粘附素大小在48至302个氨基酸之间的肽段。胶原结合需要一个代表YadA中间区域的302个氨基酸的片段。表达数百个紧密相关粘附表位的嵌合鞭毛丝为分析粘附素-受体相互作用及粘附蛋白的功能表位提供了通用工具。

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