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脂蛋白 LpqW 对于棒状杆菌周质糖脂的甘露糖基化是必不可少的。

The lipoprotein LpqW is essential for the mannosylation of periplasmic glycolipids in Corynebacteria.

机构信息

Australian Research Council Centre of Excellence in Structural and Functional Microbial Genomics, Monash University, Victoria 3800, Australia.

出版信息

J Biol Chem. 2012 Dec 14;287(51):42726-38. doi: 10.1074/jbc.M112.373415. Epub 2012 Oct 22.

DOI:10.1074/jbc.M112.373415
PMID:23091062
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3522272/
Abstract

Phosphatidylinositol mannosides (PIM), lipomannan (LM), and lipoarabinomannan (LAM) are essential components of the cell wall and plasma membrane of mycobacteria, including the human pathogen Mycobacterium tuberculosis, as well as the related Corynebacterineae. We have previously shown that the lipoprotein, LpqW, regulates PIM and LM/LAM biosynthesis in mycobacteria. Here, we provide direct evidence that LpqW regulates the activity of key mannosyltransferases in the periplasmic leaflet of the cell membrane. Inactivation of the Corynebacterium glutamicum lpqW ortholog, NCgl1054, resulted in a slow growth phenotype and a global defect in lipoglycan biosynthesis. The NCgl1054 mutant lacked LAMs and was defective in the elongation of the major PIM species, AcPIM2, as well as a second glycolipid, termed Gl-X (mannose-α1-4-glucuronic acid-α1-diacylglycerol), which function as membrane anchors for LM-A and LM-B, respectively. Elongation of AcPIM2 and Gl-X was found to be dependent on expression of polyprenol phosphomannose (ppMan) synthase. However, the ΔNCgl1054 mutant synthesized normal levels of ppMan, indicating that LpqW is not required for synthesis of this donor. A spontaneous suppressor strain was isolated in which lipoglycan synthesis in the ΔNCgl1054 mutant was partially restored. Genome-wide sequencing indicated that a single amino acid substitution within the ppMan-dependent mannosyltransferase MptB could bypass the need for LpqW. Further evidence of an interaction is provided by the observation that MptB activity in cell-free extracts was significantly reduced in the absence of LpqW. Collectively, our results suggest that LpqW may directly activate MptB, highlighting the role of lipoproteins in regulating key cell wall biosynthetic pathways in these bacteria.

摘要

磷脂酰肌醇甘露糖 (PIM)、脂甘露聚糖 (LM) 和脂阿拉伯甘露聚糖 (LAM) 是分枝杆菌细胞壁和质膜的重要组成部分,包括人类病原体结核分枝杆菌以及相关的棒状杆菌。我们之前已经表明,脂蛋白 LpqW 调节分枝杆菌中的 PIM 和 LM/LAM 生物合成。在这里,我们提供了直接的证据表明 LpqW 调节质膜周质小叶中关键甘露糖基转移酶的活性。失活谷氨酸棒状杆菌的 NCgl1054 同源物,NCgl1054,导致生长缓慢表型和脂聚糖生物合成的全局缺陷。NCgl1054 突变体缺乏 LAMs 并且在主要 PIM 物种 AcPIM2 的伸长以及第二种糖脂,称为 Gl-X(甘露糖-α1-4-葡萄糖醛酸-α1-二酰基甘油),分别作为 LM-A 和 LM-B 的膜锚,存在缺陷。发现 AcPIM2 和 Gl-X 的伸长依赖于多萜醇磷酸甘露糖 (ppMan) 合酶的表达。然而,ΔNCgl1054 突变体合成正常水平的 ppMan,表明 LpqW 不是该供体合成所必需的。分离出一个自发的抑制子菌株,其中ΔNCgl1054 突变体中的脂聚糖合成部分恢复。全基因组测序表明,ppMan 依赖性甘露糖基转移酶 MptB 中的单个氨基酸取代可以绕过对 LpqW 的需求。观察到在没有 LpqW 的情况下细胞提取物中 MptB 活性显着降低,这提供了进一步的相互作用证据。总之,我们的结果表明 LpqW 可能直接激活 MptB,突出了脂蛋白在调节这些细菌中关键细胞壁生物合成途径中的作用。

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