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首页> 外文期刊>Molecular Microbiology >Genome-wide analysis of transcriptional hierarchy and feedback regulation in the flagellar system of Helicobacter pylori.
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Genome-wide analysis of transcriptional hierarchy and feedback regulation in the flagellar system of Helicobacter pylori.

机译:幽门螺杆菌鞭毛系统中转录层次和反馈调控的全基因组分析。

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摘要

The flagellar system of Helicobacter pylori, which comprises more than 40 mostly unclustered genes, is essential for colonization of the human stomach mucosa. In order to elucidate the complex transcriptional circuitry of flagellar biosynthesis in H. pylori and its link to other cell functions, mutants in regulatory genes governing flagellar biosynthesis (rpoN, flgR, flhA, flhF, HP0244) and whole-genome microarray technology were used in this study. The regulon controlled by RpoN, its activator FlgR (FleR) and the cognate histidine kinase HP0244 (FleS) was characterized on a genome-wide scale for the first time. Seven novel genes (HP1076, HP1233, HP1154/1155, HP0366/367, HP0869) were identified as belonging to RpoN-associated flagellar regulons. The hydrogenase accessory gene HP0869 was the only annotated non-flagellar gene in the RpoN regulon. Flagellar basal body components FlhA and FlhF were characterized as functional equivalents to master regulators in H. pylori, as their absence led to a general reduction of transcripts in the RpoN (class 2) and FliA (class 3) regulons, and of 24 genes newly attributed to intermediate regulons, under the control of two or more promoters. FlhA- and FlhF-dependent regulons comprised flagellar and non-flagellar genes. Transcriptome analysis revealed that negative feedback regulation of the FliA regulon was dependent on the antisigma factor FlgM. FlgM was also involved in FlhA- but not FlhF-dependent feedback control of the RpoN regulon. In contrast to other bacteria, chemotaxis and flagellar motor genes were not controlled by FliA or RpoN. A true master regulator of flagellar biosynthesis is absent in H. pylori, consistent with the essential role of flagellar motility and chemotaxis for this organism.
机译:幽门螺杆菌的鞭毛系统,包含40多个大部分未聚类的基因,对于人类胃粘膜的定殖至关重要。为了阐明幽门螺杆菌鞭毛生物合成的复杂转录途径及其与其他细胞功能的联系,在调控鞭毛生物合成的调节基因中的突变体(rpoN,flgR,fhlA,fhlF,HP0244)和全基因组微阵列技术被用于这项研究。由RpoN,其激活因子FlgR(FleR)和相关组氨酸激酶HP0244(FleS)控制的调节子首次在全基因组范围内进行了表征。七个新基因(HP1076,HP1233,HP1154 / 1155,HP0366 / 367,HP0869)被鉴定为属于RpoN相关的鞭毛调节子。氢化酶辅助基因HP0869是RpoN调节子中唯一注释的非鞭毛基因。鞭毛基体成分FlhA和FlhF被表征为幽门螺杆菌中主要调控子的功能等同物,因为它们的缺失导致RpoN(2类)和FliA(3类)调节子的转录物普遍减少,并且新发现了24个基因在两个或多个启动子的控制下归因于中间调节子。 FlhA和FlhF依赖的调控子包含鞭毛和非鞭毛基因。转录组分析显示,FliA调节子的负反馈调节取决于抗西格玛因子FlgM。 FlgM还参与了RpoN调节子的FlhA依赖性但不依赖FlhF的反馈控制。与其他细菌相反,趋化性和鞭毛运动基因不受FliA或RpoN的控制。幽门螺杆菌中没有真正的鞭毛生物合成的主调节剂,这与该生物的鞭毛运动性和趋化性的基本作用是一致的。

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