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新月柄杆菌中过氧化氢酶-过氧化物酶 KatG 的调控依赖于 OxyR 而不依赖于 Fur。

Regulation of catalase-peroxidase KatG is OxyR dependent and Fur independent in Caulobacter crescentus.

机构信息

Departamento de Microbiologia, Instituto de Ciências Biomédicas, Universidade de São Paulo, Av. Prof. Lineu Prestes 1374, 05508-000 São Paulo, SP, Brazil.

出版信息

J Bacteriol. 2011 Apr;193(7):1734-44. doi: 10.1128/JB.01339-10. Epub 2011 Jan 21.

Abstract

Most organisms that grow in the presence of oxygen possess catalases and/or peroxidases, which are necessary for scavenging the H(2)O(2) produced by aerobic metabolism. In this work we investigate the pathways that regulate the Caulobacter crescentus katG gene, encoding the only enzyme with catalase-peroxidase function in this bacterium. The transcriptional start site of the katG gene was determined, showing a short 5' untranslated region. The katG regulatory region was mapped by serial deletions, and the results indicate that there is a single promoter, which is responsible for induction at stationary phase. An oxyR mutant strain was constructed; it showed decreased katG expression, and no KatG protein or catalase-peroxidase activity was detected in stationary-phase cell extracts, implying that OxyR is the main positive regulator of the C. crescentus katG gene. Purified OxyR protein bound to the katG regulatory region between nucleotides -42 and -91 from the transcription start site, as determined by a DNase I footprinting assay, and a canonical OxyR binding site was found in this region. Moreover, OxyR binding was shown to be redox dependent, given that only oxidized proteins bound adjacent to the -35 sequence of the promoter and the katG P1 promoter was activated by OxyR in an H(2)O(2)-dependent manner. On the other hand, this work showed that the iron-responsive regulator Fur does not regulate C. crescentus katG, since a fur mutant strain presented wild-type levels of katG transcription and catalase-peroxidase production and activity, and the purified Fur protein was not able to bind to the katG regulatory region.

摘要

大多数在氧气存在下生长的生物体都拥有过氧化氢酶和/或过氧化物酶,这些酶对于清除有氧代谢产生的 H(2)O(2)是必需的。在这项工作中,我们研究了调节新月柄杆菌 katG 基因的途径,该基因编码该细菌中唯一具有过氧化氢酶-过氧化物酶功能的酶。确定了 katG 基因的转录起始位点,显示出短的 5'非翻译区。通过连续缺失来映射 katG 调控区,结果表明存在一个单一的启动子,该启动子负责在静止期诱导。构建了 oxyR 突变株;它显示出 katG 表达减少,并且在静止期细胞提取物中未检测到 KatG 蛋白或过氧化氢酶-过氧化物酶活性,这意味着 OxyR 是 C. crescentus katG 基因的主要正调控因子。通过 DNase I 足迹测定实验,确定纯化的 OxyR 蛋白与转录起始位点上游的核苷酸 -42 至 -91 之间的 katG 调控区结合,并且在该区域发现了一个典型的 OxyR 结合位点。此外,OxyR 结合被证明是氧化还原依赖性的,因为只有氧化的蛋白质与启动子的-35 序列相邻结合,并且 OxyR 以 H(2)O(2)依赖的方式激活 katG P1 启动子。另一方面,这项工作表明铁反应调节因子 Fur 不调节新月柄杆菌 katG,因为 fur 突变株表现出野生型 katG 转录和过氧化氢酶-过氧化物酶的产生和活性,并且纯化的 Fur 蛋白不能与 katG 调控区结合。

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