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枯草芽孢杆菌依赖叶酸的 tRNA 甲基转移酶稳定的催化中间体和几种黄素氧化还原态。

A catalytic intermediate and several flavin redox states stabilized by folate-dependent tRNA methyltransferase from Bacillus subtilis.

机构信息

Centre de Recherche de Gif, CNRS, 91198 Gif-sur-Yvette, France.

出版信息

Biochemistry. 2011 Jun 14;50(23):5208-19. doi: 10.1021/bi1019463. Epub 2011 May 18.

DOI:10.1021/bi1019463
PMID:21561081
Abstract

The flavoprotein TrmFO catalyzes the C5 methylation of uridine 54 in the TΨC loop of tRNAs using 5,10-methylenetetrahydrofolate (CH(2)THF) as a methylene donor and FAD as a reducing agent. Here, we report biochemical and spectroscopic studies that unravel the remarkable capability of Bacillus subtilis TrmFO to stabilize, in the presence of oxygen, several flavin-reduced forms, including an FADH(•) radical, and a catalytic intermediate endowed with methylating activity. The FADH(•) radical was characterized by high-field electron paramagnetic resonance and electron nuclear double-resonance spectroscopies. Interestingly, the enzyme exhibited tRNA methylation activity in the absence of both an added carbon donor and an external reducing agent, indicating that a reaction intermediate, containing presumably CH(2)THF and FAD hydroquinone, is present in the freshly purified enzyme. Isolation by acid treatment, under anaerobic conditions, of noncovalently bound molecules, followed by mass spectrometry analysis, confirmed the presence in TrmFO of nonmodified FAD. Addition of formaldehyde to the purified enzyme protects the reduced flavins from decay by probably preventing degradation of CH(2)THF. The absence of air-stable reduced FAD species during anaerobic titration of oxidized TrmFO, performed in the absence or presence of added CH(2)THF, argues against their thermodynamic stabilization but rather implicates their kinetic trapping by the enzyme. Altogether, the unexpected isolation of a stable catalytic intermediate suggests that the flavin-binding pocket of TrmFO is a highly insulated environment, diverting the reduced FAD present in this intermediate from uncoupled reactions.

摘要

黄素蛋白 TrmFO 使用 5,10-亚甲基四氢叶酸 (CH(2)THF) 作为亚甲基供体和 FAD 作为还原剂,催化 tRNA 的 TΨC 环中尿嘧啶 54 的 C5 甲基化。在这里,我们报告了生化和光谱研究,揭示了枯草芽孢杆菌 TrmFO 的非凡能力,即在氧气存在下,稳定几种黄素还原形式,包括 FADH(•)自由基和具有甲基化活性的催化中间物。FADH(•)自由基通过高磁场电子顺磁共振和电子-核双共振光谱学进行了表征。有趣的是,该酶在没有外加碳供体和外部还原剂的情况下表现出 tRNA 甲基化活性,表明在新鲜纯化的酶中存在可能含有 CH(2)THF 和 FAD 氢醌的反应中间物。在厌氧条件下通过酸处理分离非共价结合的分子,并通过质谱分析,证实了 TrmFO 中存在非修饰的 FAD。向纯化酶中添加甲醛可能通过防止 CH(2)THF 降解来保护还原黄素不衰减。在没有或有外加 CH(2)THF 的情况下,对氧化 TrmFO 进行厌氧滴定时,未观察到稳定的还原 FAD 物质,这表明它们不是热力学稳定的,而是可能被酶动力学捕获。总之,出乎意料地分离出稳定的催化中间物表明,TrmFO 的黄素结合口袋是一个高度隔离的环境,将存在于该中间物中的还原 FAD 从无偶联反应中转移出来。

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