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The crystal structure of the transcriptional regulator HucR from Deinococcus radiodurans reveals a repressor preconfigured for DNA binding

机译:放射嗜热球菌(Deinococcus radiodurans)转录调节因子HucR的晶体结构揭示了阻遏物已预先配置用于DNA结合

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摘要

We report here the 2.3 angstrom resolution structure of the hypothetical uricase regulator (HucR) from Deinococcus radiodurans R1. HucR, a member of the MarR family of DNA-binding proteins, was previously shown to repress its own expression as well as that of a uricase, a repression that is alleviated both in vivo and in vitro upon binding uric acid, the substrate for uricase. As uric acid is a potent scavenger of reactive oxygen species, and as D. radiodurans is known for its remarkable resistance to DNA-damaging agents, these observations indicate a novel oxidative stress response mechanism. The crystal structure of HucR in the absence of ligand or DNA reveals a dimer in which the DNA recognition helices are preconfigured for DNA binding. This configuration of DNA-binding domains is achieved through an apparently stable dimer interface that, in contrast to what is observed in other MarR homologs for which structures have been determined, shows little conformational heterogeneity in the absence of ligand. An additional amino-terminal segment, absent from other MarR homologs, appears to brace the principal helix of the dimerization interface. However, although HucR is preconfigured for DNA binding, the presence of a stacked pair of symmetry-related histidine residues at a central pivot point in the dimer interface suggests a mechanism for a conformational change to attenuate DNA binding. (c) 2006 Elsevier Ltd. All rights reserved.
机译:我们在这里报告的Deinococcus radiodurans R1假设的尿酸酶调节剂(HucR)的2.3埃分辨率结构。 HucR是MarR DNA结合蛋白家族的成员,先前已证明它能抑制自身的表达以及尿酸酶的表达,这种抑制作用会在结合尿酸(尿酸酶的底物)后在体内和体外缓解。 。由于尿酸是一种有效的活性氧清除剂,而放射性杜鹃(D.radiusdurans)以其对DNA破坏剂的卓越抗性而闻名,这些发现表明了一种新颖的氧化应激反应机制。在不存在配体或DNA的情况下,HucR的晶体结构揭示了一个二聚体,其中DNA识别螺旋被预先配置用于DNA结合。 DNA结合结构域的这种配置是通过表面上稳定的二聚体界面实现的,该界面与在已确定结构的其他MarR同源物中观察到的相反,在没有配体的情况下几乎没有构象异质性。其他MarR同系物不存在的另一个氨基末端片段似乎支撑了二聚化界面的主要螺旋结构。但是,尽管HucR已预先配置为可与DNA结合,但是在二聚体界面的中心枢轴点处存在一对堆叠的对称相关组氨酸残基,提示存在构象变化可减弱DNA结合的机制。 (c)2006 Elsevier Ltd.保留所有权利。

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