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聚异戊二烯单磷酸甘露糖合酶Cg-Ppm1的破坏以及谷氨酸棒杆菌中无脂多糖突变体的产生。

Disruption of Cg-Ppm1, a polyprenyl monophosphomannose synthase, and the generation of lipoglycan-less mutants in Corynebacterium glutamicum.

作者信息

Gibson Kevin J C, Eggeling Lothar, Maughan William N, Krumbach Karin, Gurcha Sudagar S, Nigou Jérôme, Puzo Germain, Sahm Hermann, Besra Gurdyal S

机构信息

School of Biosciences, University of Birmingham, Edgbaston, Birmingham B15 2TT, United Kingdom.

出版信息

J Biol Chem. 2003 Oct 17;278(42):40842-50. doi: 10.1074/jbc.M307988200. Epub 2003 Aug 6.

DOI:10.1074/jbc.M307988200
PMID:12904287
Abstract

The glycosyl donor, polyprenyl monophosphomannose (PPM), has been shown to be involved in the biosynthesis of the mycobacterial lipoglycans: lipomannan and lipoarabinomannan. The mycobacterial PPM synthase (Mt-ppm1) catalyzes the transfer of mannose from GDP-mannose to polyprenyl phosphates. Based on sequence homology to Mt-ppm1, we have identified the PPM synthase from Corynebacterium glutamicum. In the present study, we demonstrate that the corynebacterial synthase is composed of two distinct domains; a catalytic domain (Cg-ppm1) and a membrane domain (Cg-ppm2). Through the inactivation of Cg-ppm1, we observed a complex phenotype that included altered cell growth rate and inability to synthesize PPM molecules and lipoglycans. When Cg-ppm2 was deleted, no observable phenotype was noted, indicating the clear organization of the two domains. The complementation of the inactivated Cg-ppm1 strain with the corresponding mycobacterial enzyme (Mt-Ppm1/D2) led to the restoration of a wild type phenotype. The present study illustrates, for the first time, the generation of a lipoglycan-less mutant based on a molecular strategy in a member of the Corynebacterianeae family. Lipoglycans are important immunomodulatory molecules involved in determining the outcome of infection, and so the generation of defined mutants and their subsequent immunological characterization is timely.

摘要

糖基供体聚异戊二烯单磷酸甘露糖(PPM)已被证明参与分枝杆菌脂糖(脂甘露聚糖和脂阿拉伯甘露聚糖)的生物合成。分枝杆菌PPM合酶(Mt-ppm1)催化甘露糖从GDP-甘露糖转移至聚异戊二烯磷酸酯。基于与Mt-ppm1的序列同源性,我们鉴定出了谷氨酸棒杆菌的PPM合酶。在本研究中,我们证明棒杆菌合酶由两个不同结构域组成:一个催化结构域(Cg-ppm1)和一个膜结构域(Cg-ppm2)。通过使Cg-ppm1失活,我们观察到一种复杂的表型,包括细胞生长速率改变以及无法合成PPM分子和脂糖。当删除Cg-ppm2时,未观察到明显表型,这表明这两个结构域的组织清晰。用相应的分枝杆菌酶(Mt-Ppm1/D2)对失活的Cg-ppm1菌株进行互补,导致野生型表型得以恢复。本研究首次说明了基于分子策略在棒杆菌科成员中产生无脂糖突变体的情况。脂糖是参与决定感染结果的重要免疫调节分子,因此生成特定突变体并对其进行后续免疫特性分析是适时的。

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