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PelA和PelB蛋白形成一种修饰和分泌复合体,这对于在……中依赖Pel多糖的生物膜形成至关重要。

PelA and PelB proteins form a modification and secretion complex essential for Pel polysaccharide-dependent biofilm formation in .

作者信息

Marmont Lindsey S, Whitfield Gregory B, Rich Jacquelyn D, Yip Patrick, Giesbrecht Laura B, Stremick Carol A, Whitney John C, Parsek Matthew R, Harrison Joe J, Howell P Lynne

机构信息

From the Program in Molecular Medicine, The Hospital for Sick Children, Toronto, Ontario M5G 0A4, Canada.

the Department of Biochemistry, University of Toronto, Toronto, Ontario M5S 1A8, Canada.

出版信息

J Biol Chem. 2017 Nov 24;292(47):19411-19422. doi: 10.1074/jbc.M117.812842. Epub 2017 Sep 27.

Abstract

The pellicle (PEL) polysaccharide is synthesized by the opportunistic pathogen and is an important biofilm constituent critical for bacterial virulence and persistence. PEL is a cationic polymer that promotes cell-cell interactions within the biofilm matrix through electrostatic interactions with extracellular DNA. Translocation of PEL across the outer membrane is proposed to occur via PelB, a membrane-embedded porin with a large periplasmic domain predicted to contain 19 tetratricopeptide repeats (TPRs). TPR-containing domains are typically involved in protein-protein interactions, and we therefore sought to determine whether PelB serves as a periplasmic scaffold that recruits other components of the PEL secretion apparatus. In this study, we show that the TPR domain of PelB interacts with PelA, an enzyme with PEL deacetylase and hydrolase activities. Structure determination of PelB TPRs 8-11 enabled us to design systematic deletions of individual TPRs and revealed that repeats 9-14, which are required for the cellular localization of PelA with PelB are also essential for PEL-dependent biofilm formation. Copurification experiments indicated that the interaction between PelA and PelB is direct and that the deacetylase activity of PelA increases and its hydrolase activity decreases when these proteins interact. Combined, our results indicate that the TPR-containing domain of PelB localizes PelA to the PEL secretion apparatus within the periplasm and that this may allow for efficient deacetylation of PEL before its export from the cell.

摘要

菌膜多糖(PEL)由机会致病菌合成,是生物膜的重要组成部分,对细菌的毒力和持久性至关重要。PEL是一种阳离子聚合物,通过与细胞外DNA的静电相互作用促进生物膜基质内的细胞间相互作用。据推测,PEL通过PelB跨外膜转运,PelB是一种膜嵌入孔蛋白,其大的周质结构域预计含有19个四肽重复序列(TPR)。含TPR的结构域通常参与蛋白质-蛋白质相互作用,因此我们试图确定PelB是否作为一种周质支架招募PEL分泌装置的其他成分。在本研究中,我们表明PelB的TPR结构域与具有PEL脱乙酰酶和水解酶活性的酶PelA相互作用。对PelB的TPR 8-11进行结构测定使我们能够设计单个TPR的系统缺失,并揭示PelA与PelB细胞定位所需的重复序列9-14对于PEL依赖性生物膜形成也至关重要。共纯化实验表明,PelA与PelB之间的相互作用是直接 的,并且当这些蛋白质相互作用时,PelA的脱乙酰酶活性增加而其水解酶活性降低。综合来看,我们的结果表明,PelB的含TPR结构域将PelA定位于周质内的PEL分泌装置,这可能允许PEL在从细胞输出之前进行有效的脱乙酰化。

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