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A DNA Region Recognized by the Nitric Oxide-Responsive Transcriptional Activator NorR Is Conserved in β- and γ-Proteobacteria

机译:一氧化氮反应性转录激活因子NorR识别的DNA区域在β和γ变形杆菌中是保守的。

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摘要

The σ54-dependent regulator NorR activates transcription of target genes in response to nitric oxide (NO) or NO-generating agents. In Ralstonia eutropha H16, NorR activates transcription of the dicistronic norAB operon that encodes NorA, a protein of unknown function, and NorB, a nitric oxide reductase. A constitutively activating NorR derivative (NorR′), in which the N-terminal signaling domain was replaced by MalE, specifically bound to the norAB upstream region as revealed by gel retardation analysis. Within a 73-bp DNA segment protected by MalE-NorR′ in a DNase I footprint assay, three conserved inverted repeats, GGT-(N7)-ACC (where N is any base), that we consider to be NorR-binding boxes were identified. Mutations altering the spacing or the base sequence of these repeats resulted in an 80 to 90% decrease of transcriptional activation by wild-type NorR. Genome database analyses demonstrate that the GT-(N7)-AC core of the inverted repeat is found in several proteobacteria upstream of gene loci encoding proteins of nitric oxide metabolism, including nitric oxide reductase (NorB), flavorubredoxin (NorV), NO dioxygenase (Hmp), and hybrid cluster protein (Hcp).
机译:依赖于σ 54 的调节子NorR响应一氧化氮(NO)或NO产生剂激活靶基因的转录。在Ralstonia eutropha H16中,NorR激活双顺反子norAB操纵子的转录,该操纵子编码功能未知的蛋白NorA和一氧化氮还原酶NorB。组成性活化的NorR衍生物(NorR'),其中N端信号域被MalE取代,特异性结合到norAB上游区域,如凝胶阻滞分析所揭示。在DNase I足迹分析中由MalE-NorR'保护的73 bp DNA片段中,我们认为是NorR结合盒的三个保守反向重复序列GGT-(N7)-ACC(其中N为任何碱基)是确定。改变这些重复序列的间隔或碱基序列的突变导致野生型NorR的转录激活降低80%至90%。基因组数据库分析表明,反向重复序列的GT-(N7)-AC核心存在于编码一氧化氮代谢蛋白的基因位点上游的几个变形杆菌中,包括一氧化氮还原酶(NorB),四氧化二氮合酶(NorV),一氧化氮( Hmp)和杂交簇蛋白(Hcp)。

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