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肉桂链霉菌中聚醚抗生素莫能菌素生物合成基因簇的分析以及monB和monC基因在氧化环化中的作用证据。

Analysis of the biosynthetic gene cluster for the polyether antibiotic monensin in Streptomyces cinnamonensis and evidence for the role of monB and monC genes in oxidative cyclization.

作者信息

Oliynyk Markiyan, Stark Christian B W, Bhatt Apoorva, Jones Michelle A, Hughes-Thomas Zoë A, Wilkinson Christopher, Oliynyk Zoryana, Demydchuk Yuliya, Staunton James, Leadlay Peter F

机构信息

Cambridge Centre for Molecular Recognition, University of Cambridge, 80 Tennis Court Road, Cambridge, CB2 1GA, UK.

出版信息

Mol Microbiol. 2003 Sep;49(5):1179-90. doi: 10.1046/j.1365-2958.2003.03571.x.

Abstract

The analysis of a candidate biosynthetic gene cluster (97 kbp) for the polyether ionophore monensin from Streptomyces cinnamonensis has revealed a modular polyketide synthase composed of eight separate multienzyme subunits housing a total of 12 extension modules, and flanked by numerous other genes for which a plausible function in monensin biosynthesis can be ascribed. Deletion of essentially all these clustered genes specifically abolished monensin production, while overexpression in S. cinnamonensis of the putative pathway-specific regulatory gene monR led to a fivefold increase in monensin production. Experimental support is presented for a recently-proposed mechanism, for oxidative cyclization of a linear polyketide intermediate, involving four enzymes, the products of monBI, monBII, monCI and monCII. In frame deletion of either of the individual genes monCII (encoding a putative cyclase) or monBII (encoding a putative novel isomerase) specifically abolished monensin production. Also, heterologous expression of monCI, encoding a flavin-linked epoxidase, in S. coelicolor was shown to significantly increase the ability of S. coelicolor to epoxidize linalool, a model substrate for the presumed linear polyketide intermediate in monensin biosynthesis.

摘要

对来自肉桂链霉菌的聚醚离子载体莫能菌素的一个候选生物合成基因簇(97千碱基对)进行分析后发现,它是一个模块化聚酮合酶,由八个独立的多酶亚基组成,共包含12个延伸模块,两侧还有许多其他基因,这些基因在莫能菌素生物合成中可能具有合理的功能。基本上删除所有这些成簇基因会特异性地消除莫能菌素的产生,而在肉桂链霉菌中过表达假定的途径特异性调控基因monR会导致莫能菌素产量增加五倍。针对最近提出的一种机制提供了实验支持,该机制涉及线性聚酮中间体的氧化环化,涉及四种酶,即monBI、monBII、monCI和monCII的产物。单独缺失monCII(编码一种假定的环化酶)或monBII(编码一种假定的新型异构酶)中的任何一个基因会特异性地消除莫能菌素的产生。此外,在天蓝色链霉菌中异源表达编码黄素连接环氧化酶的monCI,结果表明天蓝色链霉菌氧化芳樟醇(莫能菌素生物合成中假定的线性聚酮中间体的模型底物)的能力显著增强。

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