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通过三种不同的机制将 TolA 蛋白募集到大肠杆菌的细胞收缩部位,以及 FtsWI 活性在募集 TolA 和 TolQ 中的关键作用。

Recruitment of the TolA Protein to Cell Constriction Sites in Escherichia coli via Three Separate Mechanisms, and a Critical Role for FtsWI Activity in Recruitment of both TolA and TolQ.

机构信息

Department of Molecular Biology and Microbiology, School of Medicine, Case Western Reserve University, Cleveland, Ohio, USA.

出版信息

J Bacteriol. 2022 Jan 18;204(1):e0046421. doi: 10.1128/JB.00464-21. Epub 2021 Nov 8.

Abstract

The Tol-Pal system of Gram-negative bacteria helps maintain the integrity of the cell envelope and ensures that invagination of the envelope layers during cell fission occurs in a well-coordinated manner. In Escherichia coli, the five Tol-Pal proteins (TolQ, -R, -A, and -B and Pal) accumulate at cell constriction sites in a manner that normally requires the activity of the cell constriction initiation protein FtsN. While septal recruitment of TolR, TolB, and Pal also requires the presence of TolQ and/or TolA, the latter two can recognize constriction sites independently of the other system proteins. What attracts TolQ or TolA to these sites is unclear. We show that FtsN indirectly attracts both proteins and that PBP1A, PBP1B, and CpoB are dispensable for their septal recruitment. However, the β-lactam aztreonam readily interferes with the septal accumulation of both TolQ and TolA, indicating that FtsN-stimulated production of septal peptidoglycan by the FtsWI synthase is critical to their recruitment. We also discovered that each of TolA's three domains can separately recognize division sites. Notably, the middle domain (TolAII) is responsible for directing TolA to constriction sites in the absence of other Tol-Pal proteins and CpoB, while recruitment of TolAI requires TolQ and that of TolAIII requires a combination of TolB, Pal, and CpoB. Additionally, we describe the construction and use of functional fluorescent sandwich fusions of the ZipA division protein, which should be more broadly valuable in future studies of the E. coli cell division machinery. Cell division (cytokinesis) is a fundamental biological process that is incompletely understood for any organism. Division of bacterial cells relies on a ring-like machinery called the septal ring or divisome that assembles along the circumference of the mother cell at the site where constriction will eventually occur. In the well-studied bacterium Escherichia coli, this machinery contains over 30 distinct proteins. We studied how two such proteins, TolA and TolQ, which also play a role in maintaining the integrity of the outer membrane, are recruited to the machinery. We find that TolA can be recruited by three separate mechanisms and that both proteins rely on the activity of a well-studied cell division enzyme for their recruitment.

摘要

革兰氏阴性菌的 Tol-Pal 系统有助于维持细胞包膜的完整性,并确保在细胞分裂过程中包膜层的内陷以协调的方式发生。在大肠杆菌中,五个 Tol-Pal 蛋白(TolQ、-R、-A、-B 和 Pal)以一种通常需要细胞收缩起始蛋白 FtsN 活性的方式在细胞收缩部位积累。虽然隔室招募 TolR、TolB 和 Pal 也需要 TolQ 和/或 TolA 的存在,但后两者可以独立于其他系统蛋白识别收缩部位。是什么吸引 TolQ 或 TolA 到这些部位尚不清楚。我们表明,FtsN 间接吸引这两种蛋白,并且 PBP1A、PBP1B 和 CpoB 对于它们的隔室募集是可有可无的。然而,β-内酰胺氨曲南很容易干扰 TolQ 和 TolA 的隔室积累,表明 FtsN 刺激的 FtsWI 合酶产生隔室肽聚糖对它们的募集至关重要。我们还发现 TolA 的三个结构域中的每一个都可以分别识别分裂位点。值得注意的是,中间结构域(TolAII)负责在没有其他 Tol-Pal 蛋白和 CpoB 的情况下将 TolA 引导到收缩部位,而 TolAI 的募集需要 TolQ,而 TolAIII 的募集需要 TolB、Pal 和 CpoB 的组合。此外,我们描述了 ZipA 分裂蛋白的功能性荧光三明治融合的构建和使用,这在未来大肠杆菌细胞分裂机制的研究中应该更具价值。细胞分裂(胞质分裂)是一种基本的生物过程,对于任何生物体来说都不完全清楚。细菌细胞的分裂依赖于一种称为隔膜环或分裂体的环状机械装置,该装置在母细胞的圆周上组装,在最终发生收缩的部位。在研究得很好的大肠杆菌中,该机械装置包含 30 多种不同的蛋白质。我们研究了两种这样的蛋白质,TolA 和 TolQ,它们也在维持外膜完整性方面发挥作用,是如何被招募到机械装置中的。我们发现 TolA 可以通过三种不同的机制被招募,并且这两种蛋白都依赖于一种研究得很好的细胞分裂酶的活性来被招募。

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