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保守的 DNA 结合蛋白 WhiA 参与枯草芽孢杆菌的细胞分裂。

The conserved DNA-binding protein WhiA is involved in cell division in Bacillus subtilis.

机构信息

Centre for Bacterial Cell Biology, Institute for Cell and Molecular Biosciences, Newcastle University, Newcastle, United Kingdom.

出版信息

J Bacteriol. 2013 Dec;195(24):5450-60. doi: 10.1128/JB.00507-13. Epub 2013 Oct 4.

Abstract

Bacterial cell division is a highly coordinated process that begins with the polymerization of the tubulin-like protein FtsZ at midcell. FtsZ polymerization is regulated by a set of conserved cell division proteins, including ZapA. However, a zapA mutation does not result in a clear phenotype in Bacillus subtilis. In this study, we used a synthetic-lethal screen to find genes that become essential when ZapA is mutated. Three transposon insertions were found in yvcL. The deletion of yvcL in a wild-type background had only a mild effect on growth, but a yvcL zapA double mutant is very filamentous and sick. This filamentation is caused by a strong reduction in FtsZ-ring assembly, suggesting that YvcL is involved in an early stage of cell division. YvcL is 25% identical and 50% similar to the Streptomyces coelicolor transcription factor WhiA, which induces ftsZ and is required for septation of aerial hyphae during sporulation. Using green fluorescent protein fusions, we show that YvcL localizes at the nucleoid. Surprisingly, transcriptome analyses in combination with a ChIP-on-chip assay gave no indication that YvcL functions as a transcription factor. To gain more insight into the function of YvcL, we searched for suppressors of the filamentous phenotype of a yvcL zapA double mutant. Transposon insertions in gtaB and pgcA restored normal cell division of the double mutant. The corresponding proteins have been implicated in the metabolic sensing of cell division. We conclude that YvcL (WhiA) is involved in cell division in B. subtilis through an as-yet-unknown mechanism.

摘要

细菌细胞分裂是一个高度协调的过程,始于中细胞处 tubulin 样蛋白 FtsZ 的聚合。FtsZ 聚合受一组保守的细胞分裂蛋白调节,包括 ZapA。然而,枯草芽孢杆菌中的 zapA 突变不会导致明显的表型。在这项研究中,我们使用合成致死筛选来寻找当 ZapA 突变时成为必需的基因。在 yvcL 中发现了三个转座子插入。在野生型背景中缺失 yvcL 对生长只有轻微影响,但 yvcL zapA 双突变体非常丝状和病态。这种丝状是由于 FtsZ 环组装的强烈减少引起的,表明 YvcL 参与细胞分裂的早期阶段。YvcL 与链霉菌 coelicolor 转录因子 WhiA 有 25%的相同性和 50%的相似性,WhiA 诱导 ftsZ,并在孢子形成期间空中菌丝体的分隔中是必需的。使用绿色荧光蛋白融合物,我们表明 YvcL 定位于核体。令人惊讶的是,转录组分析与 ChIP-on-chip 测定相结合没有表明 YvcL 作为转录因子发挥作用。为了更深入地了解 YvcL 的功能,我们搜索了 yvcL zapA 双突变体丝状表型的抑制剂。gtaB 和 pgcA 中的转座子插入恢复了双突变体的正常细胞分裂。相应的蛋白质已被牵连到细胞分裂的代谢感应中。我们得出结论,YvcL(WhiA)通过未知的机制参与枯草芽孢杆菌的细胞分裂。

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