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首页> 外文期刊>Molecular Microbiology >Mutational analysis of MarR, the negative regulator of marRAB expression in Escherichia coli, suggests the presence of two regions required for DNA binding.
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Mutational analysis of MarR, the negative regulator of marRAB expression in Escherichia coli, suggests the presence of two regions required for DNA binding.

机译:MarR(大肠杆菌中marRAB表达的负调节剂)的突变分析表明存在DNA结合所需的两个区域。

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摘要

MarR, the negative regulator of the Escherichia coli multiple antibiotic resistance (marRAB) operon, is a member of a newly recognized family of regulatory proteins. The amino acid sequences of these proteins do not display any apparent homologies to the DNA binding domains of prokaryotic transcription regulators and a DNA binding motif for any one of the MarR homologues is currently unknown. In order to define regions of MarR required for DNA binding, mutant repressors, selected based on their ability to interfere with (negatively complement) the activity of wild-type MarR, were isolated. As determined using gel mobility shift assays, 13 out of 14 negative complementing mutants tested were unable to bind DNA in vitro. Three negative complementing alleles presumably specify truncated repressors and one of these proteins, a 120 residue MarR, can bind DNA in vitro. Most of the negative complementing mutations were clustered within two areas of MarR with features related to a helix-turn-helix DNA binding motif. These regions are presumed to be required for the DNA binding activity of the repressor.
机译:MarR是大肠杆菌多重抗生素抗性(marRAB)操纵子的负调节剂,是新近认可的调节蛋白家族的成员。这些蛋白质的氨基酸序列与原核转录调节子的DNA结合结构域之间没有任何明显的同源性,目前还未知任何一种MarR同源物的DNA结合基序。为了定义DNA结合所需的MarR区域,分离了基于其干扰(负互补)野生型MarR活性的能力选择的突变阻遏物。如使用凝胶迁移率变动分析所确定的,测试的14个阴性互补突变体中有13个不能在体外结合DNA。推测三个负互补等位基因指定了截短的阻遏物,其中一种蛋白质,一个120个残基的MarR,可以在体外结合DNA。大多数负互补突变都聚集在MarR的两个区域内,具有与螺旋-转-螺旋-DNA结合基序有关的特征。推测这些区域是阻遏物的DNA结合活性所必需的。

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