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在大肠杆菌中,MreB和FtsZ通过需要PBP 2的独立途径指导侧细胞壁的合成。

In Escherichia coli, MreB and FtsZ direct the synthesis of lateral cell wall via independent pathways that require PBP 2.

作者信息

Varma Archana, Young Kevin D

机构信息

Department of Microbiology and Immunology, University of North Dakota School of Medicine and Health Sciences, Grand Forks, North Dakota 58202-9037, USA.

出版信息

J Bacteriol. 2009 Jun;191(11):3526-33. doi: 10.1128/JB.01812-08. Epub 2009 Apr 3.

Abstract

In Escherichia coli, the cytoplasmic proteins MreB and FtsZ play crucial roles in ensuring that new muropeptide subunits are inserted into the cell wall in a spatially correct way during elongation and division. In particular, to retain a constant diameter and overall shape, new material must be inserted into the wall uniformly around the cell's perimeter. Current thinking is that MreB accomplishes this feat through intermediary proteins that tether peptidoglycan synthases to the outer face of the inner membrane. We tested this idea in E. coli by using a DD-carboxypeptidase mutant that accumulates pentapeptides in its peptidoglycan, allowing us to visualize new muropeptide incorporation. Surprisingly, inhibiting MreB with the antibiotic A22 did not result in uneven insertion of new wall, although the cells bulged and lost their rod shapes. Instead, uneven (clustered) incorporation occurred only if MreB and FtsZ were inactivated simultaneously, providing the first evidence in E. coli that FtsZ can direct murein incorporation into the lateral cell wall independently of MreB. Inhibiting penicillin binding protein 2 (PBP 2) alone produced the same clustered phenotype, implying that MreB and FtsZ tether peptidoglycan synthases via a common mechanism that includes PBP 2. However, cell shape was determined only by the presence or absence of MreB and not by the even distribution of new wall material as directed by FtsZ.

摘要

在大肠杆菌中,细胞质蛋白MreB和FtsZ在确保新的胞壁肽亚基在伸长和分裂过程中以空间正确的方式插入细胞壁方面发挥着关键作用。特别是,为了保持恒定的直径和整体形状,必须在细胞周长周围均匀地将新物质插入细胞壁。目前的观点认为,MreB通过将肽聚糖合酶拴在内膜外表面的中间蛋白来完成这一壮举。我们通过使用一种在其肽聚糖中积累五肽的DD - 羧肽酶突变体在大肠杆菌中测试了这一想法,从而使我们能够观察到新的胞壁肽掺入情况。令人惊讶的是,用抗生素A22抑制MreB并没有导致新细胞壁的不均匀插入,尽管细胞出现肿胀并失去了杆状形态。相反,只有当MreB和FtsZ同时失活时才会发生不均匀(聚集)掺入,这为大肠杆菌中FtsZ可以独立于MreB将胞壁质掺入侧细胞壁提供了首个证据。单独抑制青霉素结合蛋白2(PBP 2)会产生相同的聚集表型,这意味着MreB和FtsZ通过包括PBP 2在内的共同机制拴系肽聚糖合酶。然而,细胞形状仅由MreB的存在与否决定,而不由FtsZ指导的新细胞壁材料的均匀分布决定。

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