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19F核磁共振揭示了MerR中金属离子和操纵基因诱导的变构效应。

19F-NMR reveals metal and operator-induced allostery in MerR.

作者信息

Song Lingyun, Teng Quincy, Phillips Robert S, Brewer John M, Summers Anne O

机构信息

Department of Microbiology, University of Georgia, Athens, GA 30602, USA.

出版信息

J Mol Biol. 2007 Aug 3;371(1):79-92. doi: 10.1016/j.jmb.2007.04.085. Epub 2007 May 10.

Abstract

Metalloregulators of the MerR family activate transcription upon metal binding by underwinding the operator-promoter DNA to permit open complex formation by pre-bound RNA polymerase. Historically, MerR's allostery has been monitored only indirectly via nuclease sensitivity or by fluorescent nucleotide probes and was very specific for Hg(II), although purified MerR binds several thiophilic metals. To observe directly MerR's ligand-induced behavior we made 2-fluorotyrosine-substituted MerR and found similar, minor changes in (19)F chemical shifts of tyrosine residues in the free protein exposed to Hg(II), Cd(II) or Zn(II). However, DNA binding elicits large chemical shift changes in MerR's tyrosine residues and in DNA-bound MerR Hg(II) provokes changes very distinct from those of Cd(II) or Zn(II). These chemical shift changes and other biophysical and phenotypic properties of wild-type MerR and relevant mutants reveal elements of an allosteric network that enables the coordination state of the metal binding site to direct metal-specific movements in the distant DNA binding site and the DNA-bound state also to affect the metal binding domain.

摘要

MerR家族的金属调节蛋白通过解开操纵子-启动子DNA来激活转录,从而允许预结合的RNA聚合酶形成开放复合物。从历史上看,MerR的变构作用仅通过核酸酶敏感性或荧光核苷酸探针间接监测,并且对Hg(II)非常特异,尽管纯化的MerR能结合几种亲硫金属。为了直接观察MerR的配体诱导行为,我们制备了2-氟酪氨酸取代的MerR,并发现暴露于Hg(II)、Cd(II)或Zn(II)的游离蛋白质中酪氨酸残基的(19)F化学位移有类似的微小变化。然而,DNA结合会引起MerR酪氨酸残基的大化学位移变化,并且在DNA结合的MerR中,Hg(II)引起的变化与Cd(II)或Zn(II)引起的变化非常不同。野生型MerR和相关突变体的这些化学位移变化以及其他生物物理和表型特性揭示了一个变构网络的元件,该网络使金属结合位点的配位状态能够指导远处DNA结合位点的金属特异性运动,并且DNA结合状态也会影响金属结合结构域。

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