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ChiZ 水平调节分枝杆菌中的细胞分裂过程。

ChiZ levels modulate cell division process in mycobacteria.

机构信息

Biomedical Research, The University of Texas Health Science Center, Tyler, TX, USA.

出版信息

Tuberculosis (Edinb). 2011 Dec;91 Suppl 1(Suppl 1):S128-35. doi: 10.1016/j.tube.2011.10.022. Epub 2011 Nov 16.

Abstract

We have previously shown that expression of chiZ (Rv2719c), encoding a cell wall hydrolase, is upregulated in response to DNA damaging agents and exposure to cephalexin. Furthermore, increased levels of ChiZ lead to decreased viability, loss of membrane integrity and defects in FtsZ-GFP localization and cell division. We now show that ChiZ N'-terminal 110 amino acid region, containing the cell wall hydrolase activity, is sufficient to modulate FtsZ-GFP localization. Further, we found that FtsZ-GFP rings are stabilized in a chiZ deletion strain indicating that ChiZ activity regulates FtsZ assembly. Overexpression of ftsZ did not reverse the reduction in viability caused by overproduction of ChiZ indicating that ChiZ neither interacts with nor directly influences FtsZ assembly. Bacterial two-hybrid assays revealed that ChiZ interacts with FtsI and FtsQ, two other septasomal proteins, but not with FtsZ. Finally, we show that ChiZ is not required for virulence of Mycobacterium tuberculosis in murine macrophages and mice. Our data suggest that optimal levels and activity of the cell wall hydrolase ChiZ are required for regulated cell division in mycobacteria.

摘要

我们之前已经表明,编码细胞壁水解酶的 chiZ(Rv2719c)的表达会对 DNA 损伤剂和头孢氨苄的暴露做出反应而上调。此外,ChiZ 水平的增加会导致细胞活力降低、膜完整性丧失以及 FtsZ-GFP 定位和细胞分裂缺陷。我们现在表明,ChiZ 的 N'-端 110 个氨基酸区域,包含细胞壁水解酶活性,足以调节 FtsZ-GFP 的定位。此外,我们发现 ChiZ 缺失菌株中的 FtsZ-GFP 环得到稳定,表明 ChiZ 活性调节 FtsZ 组装。FtsZ 的过表达并不能逆转 ChiZ 过表达导致的细胞活力降低,表明 ChiZ 既不与 FtsZ 相互作用,也不直接影响 FtsZ 组装。细菌双杂交测定表明,ChiZ 与 FtsI 和 FtsQ 相互作用,FtsI 和 FtsQ 是另两种隔膜蛋白,但与 FtsZ 不相互作用。最后,我们表明 ChiZ 不是结核分枝杆菌在鼠巨噬细胞和小鼠中毒力所必需的。我们的数据表明,细胞壁水解酶 ChiZ 的最佳水平和活性是分枝杆菌有规律的细胞分裂所必需的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5d0a/3256928/2c8a19b79816/nihms-339339-f0001.jpg

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