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毛发激活幽门螺杆菌中 2-氧戊二酸氧化还原酶基因(oorDABC)的表达。

Fur activates expression of the 2-oxoglutarate oxidoreductase genes (oorDABC) in Helicobacter pylori.

机构信息

Department of Microbiology and Immunology, Uniformed Services University of the Health Sciences, Bethesda, Maryland, USA.

出版信息

J Bacteriol. 2012 Dec;194(23):6490-7. doi: 10.1128/JB.01226-12. Epub 2012 Sep 21.

Abstract

Helicobacter pylori is a highly successful pathogen that colonizes the gastric mucosa of ∼50% of the world's population. Within this colonization niche, the bacteria encounter large fluctuations in nutrient availability. As such, it is critical that this organism regulate expression of key metabolic enzymes so that they are present when environmental conditions are optimal for growth. One such enzyme is the 2-oxoglutarate (α-ketoglutarate) oxidoreductase (OOR), which catalyzes the conversion of α-ketoglutarate to succinyl coenzyme A (succinyl-CoA) and CO(2). Previous studies from our group suggested that the genes that encode the OOR are activated by iron-bound Fur (Fe-Fur); microarray analysis showed that expression of oorD, oorA, and oorC was altered in a fur mutant strain of H. pylori. The goal of the present work was to more thoroughly characterize expression of the oorDABC genes in H. pylori as well as to define the role of Fe-Fur in this process. Here we show that these four genes are cotranscribed as an operon and that expression of the operon is decreased in a fur mutant strain. Transcriptional start site mapping and promoter analysis revealed the presence of a canonical extended -10 element but a poorly conserved -35 element upstream of the +1. Additionally, we identified a conserved Fur binding sequence ∼130 bp upstream of the transcriptional start site. Transcriptional analysis using promoter fusions revealed that this binding sequence was required for Fe-Fur-mediated activation. Finally, fluorescence anisotropy assays indicate that Fe-Fur specifically bound this Fur box with a relatively high affinity (dissociation constant [K(d)] = 200 nM). These findings provide novel insight into the genetic regulation of a key metabolic enzyme and add to our understanding of the diverse roles Fur plays in gene regulation in H. pylori.

摘要

幽门螺杆菌是一种高度成功的病原体,它定植在世界上约 50%人口的胃黏膜中。在这个定植部位,细菌会遇到营养物质可用性的巨大波动。因此,该生物体调节关键代谢酶的表达至关重要,以便在环境条件最有利于生长时存在这些酶。一种这样的酶是 2-氧戊二酸(α-酮戊二酸)氧化还原酶(OOR),它催化 α-酮戊二酸转化为琥珀酰辅酶 A(琥珀酰-CoA)和 CO2。我们小组的先前研究表明,编码 OOR 的基因被铁结合 Fur(Fe-Fur)激活;微阵列分析表明,H. pylori 的 fur 突变菌株中 oorD、oorA 和 oorC 的表达发生了改变。本工作的目的是更全面地描述 H. pylori 中 oorDABC 基因的表达情况,并确定 Fe-Fur 在这一过程中的作用。这里我们表明,这四个基因作为一个操纵子共转录,并且在 fur 突变菌株中,操纵子的表达减少。转录起始位点作图和启动子分析显示,在 +1 上游存在一个典型的扩展-10 元件,但-35 元件的保守性较差。此外,我们在转录起始位点上游约 130bp 处发现了一个保守的 Fur 结合序列。使用启动子融合进行的转录分析表明,该结合序列是 Fe-Fur 介导的激活所必需的。最后,荧光各向异性测定表明,Fe-Fur 特异性地以相对较高的亲和力(解离常数 [Kd] = 200 nM)结合这个 Fur 盒。这些发现为关键代谢酶的遗传调控提供了新的见解,并加深了我们对 Fur 在 H. pylori 基因调控中发挥的多种作用的理解。

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