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Genes involved in Sec-independent membrane targeting of hydrogenase in Azotobacter chroococcum.

机译:参与绿脓杆菌中不依赖于Sec的氢酶靶向膜的基因。

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摘要

Sec-independent translocation systems have been characterised in Escherichia coli and other bacteria and differ from the Sec-dependent system by transporting fully folded proteins using the transmembrane proton electrochemical gradient. Proteins transported by this system bear a twin-arginine motif (tat) in the N-terminal signal peptide and include several cofactor-containing proteins. Azotobacter chroococcum strain (MCD124) has a soluble hydrogenase, which exhibited low O(2)-dependent H(2) uptake, and a shift in the pH of the culture to a more alkaline range during growth. We show that the DNA region capable of complementing this strain contains the tatABC genes and that mutations in the tatA gene reproduced the soluble hydrogenase and the culture pH shift phenotypes. We also show that insertional mutation in the tatC gene at a position corresponding to its C-terminal region had no effect on hydrogenase activity, but induced the pH shift of the culture. Sequence and mutagenesis analyses of this genomic region suggest that these genes form an operon that does not contain a tatD-like gene. A mutation in hupZ of the main hup gene region, coding for a possible b-type cytochrome also yielded a soluble hydrogenase, but not the pH-shift phenotype.
机译:不依赖于Sec的转运系统已在大肠杆菌和其他细菌中得到了表征,并且与不依赖于Sec的系统通过使用跨膜质子电化学梯度转运完全折叠的蛋白质而有所不同。通过该系统转运的蛋白质在N端信号肽中带有一个双精氨酸基序(tat),并包括几种含辅因子的蛋白质。绿脓杆菌菌株(MCD124)具有可溶性的氢化酶,表现出低的O(2)依赖H(2)摄取,以及在生长过程中培养液的pH值移至更碱性的范围。我们显示,能够补充此菌株的DNA区域包含tatABC基因,并且tatA基因中的突变重现了可溶性氢化酶和培养液pH迁移表型。我们还表明,在tatC基因对应于其C端区域的位置插入突变对氢化酶活性没有影响,但诱导了培养液的pH改变。该基因组区域的序列和诱变分析表明,这些基因形成不包含tatD样基因的操纵子。 hupZ主要基因区域的hupZ突变,编码可能的b型细胞色素,也产生了可溶性氢化酶,但没有产生pH移位表型。

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