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一种假定的亚精胺合酶与鞭毛开关蛋白FliM相互作用并调节幽门螺杆菌的运动性。

A putative spermidine synthase interacts with flagellar switch protein FliM and regulates motility in Helicobacter pylori.

作者信息

Zhang Huawei, Lam Kwok Ho, Lam Wendy Wai Ling, Wong Sandra Yuen Yuen, Chan Vera Sau Fong, Au Shannon Wing Ngor

机构信息

Centre for Protein Science and Crystallography, School of Life Sciences, The Chinese University of Hong Kong, Hong Kong.

Division of Rheumatology & Clinical Immunology, Department of Medicine, Li Ka Shing Faculty of Medicine, The University of Hong Kong, Hong Kong.

出版信息

Mol Microbiol. 2017 Dec;106(5):690-703. doi: 10.1111/mmi.13829. Epub 2017 Sep 21.

DOI:10.1111/mmi.13829
PMID:28868744
Abstract

The flagellar motor is an important virulence factor in infection by many bacterial pathogens. Motor function can be modulated by chemotactic proteins and recently appreciated proteins that are not part of the flagellar or chemotaxis systems. How these latter proteins affect flagellar activity is not fully understood. Here, we identified spermidine synthase SpeE as an interacting partner of switch protein FliM in Helicobacter pylori using pull-down assay and mass spectrometry. To understand how SpeE contributes to flagellar motility, a speE-null mutant was generated and its motility behavior was evaluated. We found that deletion of SpeE did not affect flagellar formation, but induced clockwise rotation bias. We further determined the crystal structure of the FliM-SpeE complex at 2.7 Å resolution. SpeE dimer binds to FliM with micromolar binding affinity, and their interaction is mediated through the β1' and β2' region of FliM middle domain. The FliM-SpeE binding interface partially overlaps with the FliM surface that interacts with FliG and is essential for proper flagellar rotational switching. By a combination of protein sequence conservation analysis and pull-down assays using FliM and SpeE orthologues in E. coli, our data suggest that FliM-SpeE association is unique to Helicobacter species.

摘要

鞭毛马达是许多细菌病原体感染过程中的一个重要毒力因子。马达功能可由趋化蛋白以及最近发现的不属于鞭毛或趋化系统的蛋白质进行调节。这些后者的蛋白质如何影响鞭毛活性尚未完全了解。在这里,我们使用下拉分析法和质谱法鉴定出精胺合酶SpeE是幽门螺杆菌中开关蛋白FliM的相互作用伙伴。为了了解SpeE如何促进鞭毛运动,我们构建了一个speE基因缺失突变体并评估了其运动行为。我们发现SpeE的缺失不影响鞭毛形成,但会诱导顺时针旋转偏向。我们进一步以2.7 Å的分辨率确定了FliM-SpeE复合物的晶体结构。SpeE二聚体以微摩尔级的结合亲和力与FliM结合,它们的相互作用是通过FliM中间结构域的β1'和β2'区域介导的。FliM-SpeE结合界面部分重叠于与FliG相互作用且对正确的鞭毛旋转切换至关重要的FliM表面。通过蛋白质序列保守性分析以及使用大肠杆菌中的FliM和SpeE直向同源物进行下拉分析相结合,我们的数据表明FliM-SpeE结合是幽门螺杆菌属特有的。

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