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核糖体RNA甲基转移酶RumA中铁硫簇的氧化还原反应:光学和电子顺磁共振研究

Redox reactions of the iron-sulfur cluster in a ribosomal RNA methyltransferase, RumA: optical and EPR studies.

作者信息

Agarwalla Sanjay, Stroud Robert M, Gaffney Betty J

机构信息

Department of Biochemistry and Biophysics, University of California-San Francisco, San Francisco, CA 94107, USA.

出版信息

J Biol Chem. 2004 Aug 13;279(33):34123-9. doi: 10.1074/jbc.M405702200. Epub 2004 Jun 4.

Abstract

An unprecedented [4Fe-4S] iron-sulfur cluster was found in RumA, the enzyme that methylates U1939 in Escherichia coli 23 S ribosomal RNA (Agarwalla, S., Kealey, J. T., Santi, D. V., and Stroud, R. M. (2002) J. Biol. Chem. 277, 8835-8840; Lee, T. T., Agarwalla, S., and Stroud, R. M. (2004) Structure 12, 397-407). Methyltransferase reactions do not involve a redox step. To understand the structural and functional roles of the cluster in RumA, we have characterized redox reactions of the iron-sulfur cluster. As isolated aerobically, RumA exhibits a visible absorbance maximum at 390 nm and is EPR silent. It cannot be reduced by anaerobic additions of dithionite. Photoreduction by deazariboflavin/EDTA gives EPR spectra, the quantity (56% of S = 1/2 species) and details (g(av) approximately 1.96-1.93) of which indicate a 4Fe-4S cluster in the reduced RumA. Oxidation of RumA by ferricyanide leads to loss of the 390-nm band and appearance of lower intensity bands at 444 and 520 nm. EPR spectra of ferricyanide-oxidized RumA show a fraction (<8%) of the FeS cluster trapped in the 3Fe-4S form (g(av) approximately 2.011) together with unusual radical-like spectrum (g' values 2.015, 2.00, and 1.95). RumA also reacts with nitric oxide to give EPR spectra characteristic of the protein-bound iron dinitrosyl species. Oxidation of the cluster leads to its decomposition and that could be a mechanism for regulating the activity of RumA under conditions of oxidative stress in the cell. Sequence data base searches revealed that RumA homologs are widespread in various kingdoms of life and contain a conserved and unique iron-sulfur cluster binding motif, CX(5)CGGC.

摘要

在RumA(一种使大肠杆菌23S核糖体RNA中的U1939发生甲基化的酶)中发现了一种前所未有的[4Fe-4S]铁硫簇(Agarwalla, S., Kealey, J. T., Santi, D. V., and Stroud, R. M. (2002) J. Biol. Chem. 277, 8835 - 8840; Lee, T. T., Agarwalla, S., and Stroud, R. M. (2004) Structure 12, 397 - 407)。甲基转移酶反应不涉及氧化还原步骤。为了了解该簇在RumA中的结构和功能作用,我们对铁硫簇的氧化还原反应进行了表征。在有氧条件下分离得到的RumA在390nm处有一个可见吸收最大值,且电子顺磁共振(EPR)无信号。通过厌氧添加连二亚硫酸盐无法将其还原。用脱氮核黄素/乙二胺四乙酸(EDTA)进行光还原可得到EPR谱,其数量(56%的S = 1/2物种)和细节(g(av)约为1.96 - 1.93)表明还原态的RumA中存在一个4Fe-4S簇。铁氰化物对RumA的氧化导致390nm处的吸收带消失,并在444和520nm处出现强度较低的吸收带。铁氰化物氧化的RumA的EPR谱显示,一部分(<8%)的FeS簇以3Fe-4S形式(g(av)约为2.011)被困住,同时伴有不寻常的类自由基谱(g'值为2.015、2.00和1.95)。RumA还与一氧化氮反应,产生蛋白质结合的铁二亚硝基物种的特征性EPR谱。该簇的氧化导致其分解,这可能是在细胞氧化应激条件下调节RumA活性的一种机制。序列数据库搜索显示,RumA同源物广泛存在于生命的各个王国中,并包含一个保守且独特的铁硫簇结合基序CX(5)CGGC。

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