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转录调节因子MetR对DNA识别的结构基础

Structural basis for DNA recognition by the transcription regulator MetR.

作者信息

Punekar Avinash S, Porter Jonathan, Carr Stephen B, Phillips Simon E V

机构信息

Research Complex at Harwell, Rutherford Appleton Laboratory, Harwell Oxford, Didcot OX11 0FA, England.

Pfizer Ltd, Ramsgate Road, Sandwich CT13 9ND, England.

出版信息

Acta Crystallogr F Struct Biol Commun. 2016 Jun;72(Pt 6):417-26. doi: 10.1107/S2053230X16006828. Epub 2016 May 23.

Abstract

MetR, a LysR-type transcriptional regulator (LTTR), has been extensively studied owing to its role in the control of methionine biosynthesis in proteobacteria. A MetR homodimer binds to a 24-base-pair operator region of the met genes and specifically recognizes the interrupted palindromic sequence 5'-TGAA-N5-TTCA-3'. Mechanistic details underlying the interaction of MetR with its target DNA at the molecular level remain unknown. In this work, the crystal structure of the DNA-binding domain (DBD) of MetR was determined at 2.16 Å resolution. MetR-DBD adopts a winged-helix-turn-helix (wHTH) motif and shares significant fold similarity with the DBD of the LTTR protein BenM. Furthermore, a data-driven macromolecular-docking strategy was used to model the structure of MetR-DBD bound to DNA, which revealed that a bent conformation of DNA is required for the recognition helix α3 and the wing loop of the wHTH motif to interact with the major and minor grooves, respectively. Comparison of the MetR-DBD-DNA complex with the crystal structures of other LTTR-DBD-DNA complexes revealed residues that may confer operator-sequence binding specificity for MetR. Taken together, the results show that MetR-DBD uses a combination of direct base-specific interactions and indirect shape recognition of the promoter to regulate the transcription of met genes.

摘要

MetR是一种赖氨酰-tRNA合成酶类型的转录调节因子(LTTR),由于其在变形菌中甲硫氨酸生物合成控制中的作用而受到广泛研究。MetR同型二聚体与met基因的一个24个碱基对的操纵子区域结合,并特异性识别间断的回文序列5'-TGAA-N5-TTCA-3'。在分子水平上,MetR与其靶DNA相互作用的机制细节仍然未知。在这项工作中,MetR的DNA结合结构域(DBD)的晶体结构在2.16 Å分辨率下被确定。MetR-DBD采用了一种带翼螺旋-转角-螺旋(wHTH)基序,并且与LTTR蛋白BenM的DBD具有显著的折叠相似性。此外,一种数据驱动的大分子对接策略被用于模拟与DNA结合的MetR-DBD的结构,这表明DNA的弯曲构象是识别螺旋α3和wHTH基序的翼环分别与大沟和小沟相互作用所必需的。将MetR-DBD-DNA复合物与其他LTTR-DBD-DNA复合物的晶体结构进行比较,揭示了可能赋予MetR操纵子序列结合特异性的残基。综上所述,结果表明MetR-DBD利用直接的碱基特异性相互作用和启动子的间接形状识别相结合的方式来调节met基因的转录。

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