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大肠杆菌 23S rRNA 甲基转移酶 RlmG(m²G1835)的结构功能研究。

Structural insights into the function of 23S rRNA methyltransferase RlmG (m²G1835) from Escherichia coli.

机构信息

Beijing Synchrotron Radiation Facility, Institute of High Energy Physics, Chinese Academy of Sciences, Beijing 100049, People's Republic of China.

出版信息

RNA. 2012 Aug;18(8):1500-9. doi: 10.1261/rna.033407.112. Epub 2012 Jul 2.

Abstract

RlmG is a specific AdoMet-dependent methyltransferase (MTase) responsible for N²-methylation of G1835 in 23S rRNA of Escherichia coli. Methylation of m²G1835 specifically enhances association of ribosomal subunits and provides a significant advantage for bacteria in osmotic and oxidative stress. Here, the crystal structure of RlmG in complex with AdoMet and its structure in solution were determined. The structure of RlmG is similar to that of the MTase RsmC, consisting of two homologous domains: the N-terminal domain (NTD) in the recognition and binding of the substrate, and the C-terminal domain (CTD) in AdoMet-binding and the catalytic process. However, there are distinct positively charged protuberances and a distribution of conserved residues contributing to the charged surface patch, especially in the NTD of RlmG for direct binding of protein-free rRNA. The RNA-binding properties of the NTD and CTD characterized by both gel electrophoresis mobility shift assays and isothermal titration calorimetry showed that NTD could bind RNA independently and RNA binding was achieved by the NTD, accomplished by a coordinating role of the CTD. The model of the RlmG-AdoMet-RNA complex suggested that RlmG may unfold its substrate RNA in the positively charged cleft between the NTD and CTD, and then G1835 disengages from its Watson-Crick pairing with C1905 and flips out to insert into the active site. Our structure and biochemical studies provide novel insights into the catalytic mechanism of G1835 methylation.

摘要

RlmG 是一种特定的 AdoMet 依赖性甲基转移酶(MTase),负责大肠杆菌 23S rRNA 中 G1835 的 N²-甲基化。m²G1835 的甲基化特异性增强了核糖体亚基的结合,并为细菌在渗透和氧化应激中提供了显著优势。在此,确定了 RlmG 与 AdoMet 复合物的晶体结构及其溶液结构。RlmG 的结构与 MTase RsmC 相似,由两个同源结构域组成:底物识别和结合的 N 端结构域(NTD),以及 AdoMet 结合和催化过程的 C 端结构域(CTD)。然而,存在明显的正电荷突出和保守残基的分布,有助于带电荷的表面斑块,特别是在 RlmG 的 NTD 中,用于与无蛋白 rRNA 的直接结合。通过凝胶电泳迁移率变动分析和等温滴定量热法表征的 NTD 和 CTD 的 RNA 结合特性表明,NTD 可以独立地结合 RNA,并且通过 NTD 实现 RNA 结合,这是由 CTD 的协调作用完成的。RlmG-AdoMet-RNA 复合物的模型表明,RlmG 可能在 NTD 和 CTD 之间的正电荷裂缝中展开其底物 RNA,然后 G1835 与其 Watson-Crick 配对 C1905 脱离并翻转出来插入活性位点。我们的结构和生化研究为 G1835 甲基化的催化机制提供了新的见解。

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