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细胞壁合成的“肇事逃逸”现象:LpoB通过保守的变构开关与PBP1b短暂结合并激活它。

The hit-and-run of cell wall synthesis: LpoB transiently binds and activates PBP1b through a conserved allosteric switch.

作者信息

Shlosman Irina, Vettiger Andrea, Bernhardt Thomas G, Kruse Andrew C, Loparo Joseph J

出版信息

bioRxiv. 2024 Dec 14:2024.12.13.628440. doi: 10.1101/2024.12.13.628440.

Abstract

The peptidoglycan (PG) cell wall is the primary protective layer of bacteria, making the process of PG synthesis a key antibiotic target. Class A penicillin-binding proteins (aPBPs) are a family of conserved and ubiquitous PG synthases that fortify and repair the PG matrix. In gram-negative bacteria, these enzymes are regulated by outer-membrane tethered lipoproteins. However, the molecular mechanism by which lipoproteins coordinate the spatial recruitment and enzymatic activation of aPBPs remains unclear. Here we use single-molecule FRET and single-particle tracking in E. coli to show that a prototypical lipoprotein activator LpoB triggers site-specific PG synthesis by PBP1b through conformational rearrangements. Once synthesis is initiated, LpoB affinity for PBP1b dramatically decreases and it dissociates from the synthesizing enzyme. Our results suggest that transient allosteric coupling between PBP1b and LpoB directs PG synthesis to areas of low peptidoglycan density, while simultaneously facilitating efficient lipoprotein redistribution to other sites in need of fortification.

摘要

肽聚糖(PG)细胞壁是细菌的主要保护层,使得PG合成过程成为关键的抗生素作用靶点。A类青霉素结合蛋白(aPBPs)是一类保守且普遍存在的PG合成酶,可强化和修复PG基质。在革兰氏阴性菌中,这些酶受外膜锚定脂蛋白的调控。然而,脂蛋白协调aPBPs的空间募集和酶促激活的分子机制仍不清楚。在此,我们利用大肠杆菌中的单分子荧光共振能量转移和单粒子追踪技术表明,典型的脂蛋白激活剂LpoB通过构象重排触发PBP1b进行位点特异性PG合成。一旦合成开始,LpoB对PBP1b的亲和力会显著降低,并从合成酶上解离。我们的结果表明,PBP1b与LpoB之间的瞬时变构偶联将PG合成导向肽聚糖密度低的区域,同时促进脂蛋白有效地重新分布到其他需要强化的位点。

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