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变形链球菌中MetR和同型半胱氨酸对甲硫氨酸合成及摄取的调控

Control of methionine synthesis and uptake by MetR and homocysteine in Streptococcus mutans.

作者信息

Sperandio Brice, Gautier Céline, McGovern Stephen, Ehrlich Dusko S, Renault Pierre, Martin-Verstraete Isabelle, Guédon Eric

机构信息

Laboratoire de Génétique Microbienne, Institut National de la Recherche Agronomique, 78352 Jouy-en-Josas Cedex, France.

出版信息

J Bacteriol. 2007 Oct;189(19):7032-44. doi: 10.1128/JB.00703-07. Epub 2007 Aug 3.

Abstract

MetR (formerly Smu.1225), a regulator of the LysR family, controls key genes for methionine supply in Streptococcus mutans. An S. mutans metR mutant is unable to transport l-methionine and to grow in the absence of this amino acid. Accordingly, MetR activates transcription by binding to the promoter regions of two gene clusters and smu.1487, whose products are involved in methionine biosynthesis (MetEF and Smu.1487) and uptake (AtmBDE). Transcriptional activation by MetR requires the presence of a 17-bp palindromic sequence, the Met box. Base substitutions in the Met box hinder the formation of a MetR-DNA complex and abolish MetR-dependent activation, showing that Met boxes correspond to MetR recognition sites. Activation by MetR occurs in methionine-depleted medium and is rapidly triggered under nonactivating conditions by the addition of homocysteine. This intermediate of methionine biosynthesis increases the affinity of MetR for DNA in vitro and appears to be the MetR coeffector in vivo. Homocysteine plays a crucial role in methionine metabolic gene regulation by controlling MetR activity. A similar mechanism of homocysteine- and MetR-dependent control of methionine biosynthetic genes operates in S. thermophilus. These data suggest a common mechanism for the regulation of the methionine supply in streptococci. However, some streptococcal species are unable to synthesize the homocysteine coeffector. This intriguing feature is discussed in the light of comparative genomics and streptococcal ecology.

摘要

MetR(原称Smu.1225)是LysR家族的一种调控因子,控制变形链球菌中甲硫氨酸供应的关键基因。变形链球菌的metR突变体无法转运L-甲硫氨酸,且在缺乏这种氨基酸的情况下无法生长。因此,MetR通过结合两个基因簇和smu.1487的启动子区域来激活转录,其产物参与甲硫氨酸的生物合成(MetEF和Smu.1487)和摄取(AtmBDE)。MetR的转录激活需要一个17bp的回文序列,即Met框的存在。Met框中的碱基替换会阻碍MetR-DNA复合物的形成,并消除MetR依赖性激活,表明Met框对应于MetR识别位点。MetR的激活发生在甲硫氨酸耗尽的培养基中,并且在非激活条件下通过添加同型半胱氨酸可迅速触发。这种甲硫氨酸生物合成的中间产物在体外增加了MetR对DNA的亲和力,并且似乎是体内的MetR辅效应物。同型半胱氨酸通过控制MetR活性在甲硫氨酸代谢基因调控中起关键作用。嗜热链球菌中存在类似的同型半胱氨酸和MetR依赖性控制甲硫氨酸生物合成基因的机制。这些数据表明链球菌中甲硫氨酸供应调控存在共同机制。然而,一些链球菌物种无法合成同型半胱氨酸辅效应物。根据比较基因组学和链球菌生态学对这一有趣特征进行了讨论。

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