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大肠杆菌两种胱氨酸转运蛋白的生理作用及不良影响

Physiological Roles and Adverse Effects of the Two Cystine Importers of Escherichia coli.

作者信息

Chonoles Imlay Karin R, Korshunov Sergey, Imlay James A

机构信息

Department of Microbiology, University of Illinois, Urbana, Illinois, USA.

Department of Microbiology, University of Illinois, Urbana, Illinois, USA

出版信息

J Bacteriol. 2015 Dec;197(23):3629-44. doi: 10.1128/JB.00277-15. Epub 2015 Sep 8.

Abstract

UNLABELLED

When cystine is added to Escherichia coli, the bacterium becomes remarkably sensitive to hydrogen peroxide. This effect is due to enlarged intracellular pools of cysteine, which can drive Fenton chemistry. Genetic analysis linked the sensitivity to YdjN, a secondary transporter that along with the FliY-YecSC ABC system is responsible for cystine uptake. FliY-YecSC has a nanomolar Km and is essential for import of trace cystine, whereas YdjN has a micromolar Km and is the predominant importer when cystine is more abundant. Oddly, both systems are strongly induced by the CysB response to sulfur scarcity. The FliY-YecSC system can import a variety of biomolecules, including diaminopimelate; it is therefore vulnerable to competitive inhibition, presumably warranting YdjN induction under low-sulfur conditions. But the consequence is that if micromolar cystine then becomes available, the abundant YdjN massively overimports it, at >30 times the total sulfur demand of the cell. The imported cystine is rapidly reduced to cysteine in a glutathione-dependent process. This action avoids the hazard of disulfide stress, but it precludes feedback inhibition of YdjN by cystine. We conjecture that YdjN possesses no cysteine allosteric site because the isostructural amino acid serine might inappropriately bind in its place. Instead, the cell partially resolves the overaccumulation of cysteine by immediately excreting it, completing a futile import/reduction/export cycle that consumes a large amount of cellular energy. These unique, wasteful, and dangerous features of cystine metabolism are reproduced by other bacteria. We propose to rename ydjN as tcyP and fliY-yecSC as tcyJLN.

IMPORTANCE

In general, intracellular metabolite pools are kept at steady, nontoxic levels by a sophisticated combination of transcriptional and allosteric controls. Surprisingly, in E. coli allosteric control is utterly absent from the primary importer of cystine. This flaw allows massive overimport of cystine, which causes acute vulnerability to oxidative stress and is remedied only by wasteful cysteine efflux. The lack of import control may be rationalized by the unusual properties of cysteine itself. This phenomenon justifies the existence of countervailing cysteine export systems, whose purpose is otherwise hard to understand. It also highlights an unexpected link between sulfur metabolism and oxidative damage. Although this investigation focused upon E. coli, experiments confirmed that similar phenomena occur in other species.

摘要

未标记

当向大肠杆菌中添加胱氨酸时,该细菌对过氧化氢变得异常敏感。这种效应是由于细胞内半胱氨酸池扩大,这会引发芬顿化学反应。遗传分析将这种敏感性与YdjN联系起来,YdjN是一种次要转运蛋白,它与FliY - YecSC ABC系统共同负责胱氨酸的摄取。FliY - YecSC的米氏常数为纳摩尔级别,对于微量胱氨酸的导入至关重要,而YdjN的米氏常数为微摩尔级别,当胱氨酸含量较高时是主要的导入蛋白。奇怪的是,这两个系统在CysB对硫缺乏的反应中均被强烈诱导。FliY - YecSC系统可以导入多种生物分子,包括二氨基庚二酸;因此它容易受到竞争性抑制,大概这就需要在低硫条件下诱导YdjN。但结果是,如果有微摩尔级别的胱氨酸可用,大量存在的YdjN会大量过量导入,超过细胞总硫需求量的30倍以上。导入的胱氨酸在一个依赖谷胱甘肽的过程中迅速还原为半胱氨酸。这一作用避免了二硫键应激的危害,但却排除了胱氨酸对YdjN的反馈抑制。我们推测YdjN不具有半胱氨酸变构位点,因为同构氨基酸丝氨酸可能会不适当地占据其位置。相反,细胞通过立即排出半胱氨酸来部分解决半胱氨酸的过度积累问题,从而完成一个徒劳的导入/还原/排出循环,消耗大量细胞能量。胱氨酸代谢的这些独特、浪费且危险的特征在其他细菌中也有体现。我们建议将ydjN重命名为tcyP,将fliY - yecSC重命名为tcyJLN。

重要性

一般来说,细胞内代谢物池通过转录调控和变构调控的复杂组合保持在稳定、无毒的水平。令人惊讶的是,在大肠杆菌中,胱氨酸的主要导入蛋白完全缺乏变构调控。这一缺陷使得胱氨酸大量过量导入,导致对氧化应激极度敏感,只能通过浪费性的半胱氨酸外排来补救。缺乏导入控制可能是由于半胱氨酸本身的特殊性质。这种现象证明了与之抗衡的半胱氨酸输出系统存在的合理性,否则其存在目的很难理解。它还突出了硫代谢与氧化损伤之间意想不到的联系。尽管这项研究聚焦于大肠杆菌,但实验证实其他物种也会出现类似现象。

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