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一种翻译后、c-di-GMP 依赖性的调节鞭毛运动的机制。

A post-translational, c-di-GMP-dependent mechanism regulating flagellar motility.

机构信息

Department of Molecular Biology, University of Wyoming, Laramie, WY 82071, USA.

出版信息

Mol Microbiol. 2010 Jun 1;76(5):1295-305. doi: 10.1111/j.1365-2958.2010.07179.x. Epub 2010 Apr 23.

DOI:10.1111/j.1365-2958.2010.07179.x
PMID:20444091
Abstract

Elevated levels of the second messenger cyclic dimeric GMP, c-di-GMP, promote transition of bacteria from single motile cells to surface-attached multicellular communities. Here we describe a post-translational mechanism by which c-di-GMP initiates this transition in enteric bacteria. High levels of c-di-GMP induce the counterclockwise bias in Escherichia coli flagellar rotation, which results in smooth swimming. Based on co-immunoprecipitation, two-hybrid and mutational analyses, the E. coli c-di-GMP receptor YcgR binds to the FliG subunit of the flagellum switch complex, and the YcgR-FliG interaction is strengthened by c-di-GMP. The central fragment of FliG binds to YcgR as well as to FliM, suggesting that YcgR-c-di-GMP biases flagellum rotation by altering FliG-FliM interactions. The c-di-GMP-induced smooth swimming promotes trapping of motile bacteria in semi-solid media and attachment of liquid-grown bacteria to solid surfaces, whereas c-di-GMP-dependent mechanisms not involving YcgR further facilitate surface attachment. The YcgR-FliG interaction is conserved in the enteric bacteria, and the N-terminal YcgR/PilZN domain of YcgR is required for this interaction. YcgR joins a growing list of proteins that regulate motility via the FliG subunit of the flagellum switch complex, which suggests that FliG is a common regulatory entryway that operates in parallel with the chemotaxis that utilizes the FliM-entryway.

摘要

第二信使环二鸟苷酸 (c-di-GMP) 水平升高可促进细菌从单个游动细胞向附着于表面的多细胞群落的转变。在这里,我们描述了 c-di-GMP 在肠细菌中引发这种转变的一种翻译后机制。高水平的 c-di-GMP 诱导大肠杆菌鞭毛旋转的逆时针偏置,导致细菌平滑游动。基于共免疫沉淀、双杂交和突变分析,大肠杆菌 c-di-GMP 受体 YcgR 与鞭毛开关复合物的 FliG 亚基结合,c-di-GMP 增强了 YcgR-FliG 相互作用。FliG 的中央片段与 YcgR 以及 FliM 结合,表明 YcgR-c-di-GMP 通过改变 FliG-FliM 相互作用来偏置鞭毛旋转。c-di-GMP 诱导的平滑游动促进了游动细菌在半固体培养基中的捕获和液体生长细菌在固体表面的附着,而不涉及 YcgR 的 c-di-GMP 依赖性机制进一步促进了表面附着。YcgR-FliG 相互作用在肠细菌中保守,并且 YcgR 的 N 端 YcgR/PilZN 结构域是这种相互作用所必需的。YcgR 加入了越来越多的通过鞭毛开关复合物的 FliG 亚基调节运动的蛋白质列表,这表明 FliG 是一个常见的调节入口,与利用 FliM 入口的趋化作用并行运作。

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