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产肠毒素大肠杆菌CFA/I菌毛与脱唾液酸GM1的结合由次要菌毛蛋白CfaE介导。

Binding of CFA/I Pili of Enterotoxigenic Escherichia coli to Asialo-GM1 Is Mediated by the Minor Pilin CfaE.

作者信息

Madhavan T P Vipin, Riches James D, Scanlon Martin J, Ulett Glen C, Sakellaris Harry

机构信息

Menzies Health Institute Queensland, School of Medical Sciences, Griffith University, Southport, QLD, Australia.

Institute for Future Environments and School of Earth, Environmental and Biological Sciences, Queensland University of Technology, Brisbane, QLD, Australia.

出版信息

Infect Immun. 2016 Apr 22;84(5):1642-1649. doi: 10.1128/IAI.01562-15. Print 2016 May.

Abstract

CFA/I pili are representatives of a large family of related pili that mediate the adherence of enterotoxigenic Escherichia coli to intestinal epithelial cells. They are assembled via the alternate chaperone-usher pathway and consist of two subunits, CfaB, which makes up the pilus shaft and a single pilus tip-associated subunit, CfaE. The current model of pilus-mediated adherence proposes that CFA/I has two distinct binding activities; the CfaE subunit is responsible for binding to receptors of unknown structure on erythrocyte and intestinal epithelial cell surfaces, while CfaB binds to various glycosphingolipids, including asialo-GM1. In this report, we present two independent lines of evidence that, contrary to the existing model, CfaB does not bind to asialo-GM1 independently of CfaE. Neither purified CfaB subunits nor CfaB assembled into pili bind to asialo-GM1. Instead, we demonstrate that binding activity toward asialo-GM1 resides in CfaE and this is essential for pilus binding to Caco-2 intestinal epithelial cells. We conclude that the binding activities of CFA/I pili for asialo-GM1, erythrocytes, and intestinal cells are inseparable, require the same amino acid residues in CfaE, and therefore depend on the same or very similar binding mechanisms.

摘要

CFA/I菌毛是一大类相关菌毛的代表,介导产肠毒素大肠杆菌与肠道上皮细胞的黏附。它们通过交替伴侣-组装分子途径组装而成,由两个亚基组成,构成菌毛杆部的CfaB和单个与菌毛尖端相关的亚基CfaE。目前关于菌毛介导黏附的模型提出,CFA/I具有两种不同的结合活性;CfaE亚基负责与红细胞和肠道上皮细胞表面未知结构的受体结合,而CfaB则与包括脱唾液酸GM1在内的各种糖鞘脂结合。在本报告中,我们提供了两条独立的证据,与现有模型相反,CfaB不能独立于CfaE与脱唾液酸GM1结合。纯化的CfaB亚基或组装成菌毛的CfaB均不与脱唾液酸GM1结合。相反,我们证明对脱唾液酸GM1的结合活性存在于CfaE中,这对于菌毛与Caco-2肠道上皮细胞的结合至关重要。我们得出结论,CFA/I菌毛对脱唾液酸GM1、红细胞和肠道细胞的结合活性是不可分割的,在CfaE中需要相同的氨基酸残基,因此依赖于相同或非常相似的结合机制。

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