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结核分枝杆菌中脂阿拉伯甘露聚糖甲基硫代木糖封端基序的生物合成

Biosynthesis of the Methylthioxylose Capping Motif of Lipoarabinomannan in Mycobacterium tuberculosis.

作者信息

Angala Shiva Kumar, McNeil Michael R, Shi Libin, Joe Maju, Pham Ha, Zuberogoitia Sophie, Nigou Jérôme, Boot Claudia M, Lowary Todd L, Gilleron Martine, Jackson Mary

机构信息

Mycobacteria Research Laboratories, Department of Microbiology, Immunology and Pathology, Colorado State University , Fort Collins, Colorado 80523-1682, United States.

Alberta Glycomics Centre and Department of Chemistry, The University of Alberta , Edmonton, Alberta T6G 2G2, Canada.

出版信息

ACS Chem Biol. 2017 Mar 17;12(3):682-691. doi: 10.1021/acschembio.6b01071. Epub 2017 Jan 20.

Abstract

Lipoarabinomannan (LAM) is a lipoglycan found in abundant quantities in the cell envelope of all mycobacteria. The nonreducing arabinan termini of LAM display species-specific structural microheterogeneity that impacts the biological activity of the entire molecule. Mycobacterium tuberculosis, for instance, produces mannoside caps made of one to three α-(1 → 2)-Manp-linked residues that may be further substituted with an α-(1 → 4)-linked methylthio-d-xylose (MTX) residue. While the biological functions and catalytic steps leading to the formation of the mannoside caps of M. tuberculosis LAM have been well established, the biosynthetic origin and biological relevance of the MTX motif remain elusive. We here report on the discovery of a five-gene cluster dedicated to the biosynthesis of the MTX capping motif of M. tuberculosis LAM, and on the functional characterization of two glycosyltransferases, MtxS and MtxT, responsible, respectively, for the production of decaprenyl-phospho-MTX (DP-MTX) and the transfer of MTX from DP-MTX to the mannoside caps of LAM. Collectively, our NMR spectroscopic and mass spectrometric analyses of mtxS and mtxT overexpressors and knockout mutants support a biosynthetic model wherein the conversion of 5'-methylthioadenosine, which is a ubiquitous byproduct of spermidine biosynthesis, into 5'-methylthioribose-1-phosphate precedes the formation of a 5'-methylthioribose nucleotide sugar, followed by the epimerization at C-3 of the ribose residue, and the transfer of MTX from the nucleotide sugar to decaprenyl-phosphate yielding the substrate for transfer onto LAM. The conservation of the MTX biosynthetic genes in a number of Actinomycetes suggests that this discrete glycosyl substituent may be more widespread in prokaryotes than originally thought.

摘要

脂阿拉伯甘露聚糖(LAM)是一种在所有分枝杆菌细胞壁中大量存在的脂多糖。LAM的非还原阿拉伯聚糖末端表现出物种特异性的结构微异质性,这会影响整个分子的生物活性。例如,结核分枝杆菌会产生由一至三个α-(1→2)-甘露糖残基连接而成的甘露糖苷帽,这些残基可能会进一步被一个α-(1→4)-连接的甲硫基-D-木糖(MTX)残基取代。虽然导致结核分枝杆菌LAM甘露糖苷帽形成的生物学功能和催化步骤已经明确,但MTX基序的生物合成起源和生物学相关性仍然不清楚。我们在此报告发现了一个由五个基因组成的基因簇,专门负责结核分枝杆菌LAM的MTX封端基序的生物合成,并对两种糖基转移酶MtxS和MtxT进行了功能表征,它们分别负责生产癸异戊烯基磷酸-MTX(DP-MTX)以及将MTX从DP-MTX转移到LAM的甘露糖苷帽上。总体而言,我们对mtxS和mtxT过表达菌株及敲除突变体的核磁共振光谱和质谱分析支持了一种生物合成模型,即亚精胺生物合成中普遍存在的副产物5'-甲硫基腺苷先转化为5'-甲硫基核糖-1-磷酸,然后形成5'-甲硫基核糖核苷酸糖,接着核糖残基在C-3处发生差向异构化,MTX从核苷酸糖转移到癸异戊烯基磷酸上,产生转移到LAM上的底物。许多放线菌中MTX生物合成基因的保守性表明,这种离散的糖基取代基在原核生物中的分布可能比最初认为的更为广泛。

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