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对胞质和线粒体乌头酸酶与一氧化氮反应产物的电子顺磁共振研究。

An EPR investigation of the products of the reaction of cytosolic and mitochondrial aconitases with nitric oxide.

作者信息

Kennedy M C, Antholine W E, Beinert H

机构信息

Department of Biochemistry, Medical College of Wisconsin, Milwaukee, Wisconsin 53226, USA.

出版信息

J Biol Chem. 1997 Aug 15;272(33):20340-7. doi: 10.1074/jbc.272.33.20340.

DOI:10.1074/jbc.272.33.20340
PMID:9252338
Abstract

Cellular studies have indicated that some Fe-S proteins, and the aconitases in particular, are targets for nitric oxide. Specifically, NO has been implicated in the intracellular process of the conversion of active cytosolic aconitase containing a [4Fe-4S] cluster, to its apo-form which functions as an iron-regulatory protein. We have undertaken the in vitro study of the reaction of NO with purified forms of both mitochondrial and cytosolic aconitases by following enzyme activity and by observing the formation of EPR signals not shown by the original reactants. Inactivation by either NO solutions or NO-producing NONOates under anaerobic conditions is seen for both enzyme isoforms. This inactivation, which occurs in the presence or absence of substrate, is accompanied by the appearance of the g = 2.02 signals of the [3Fe-4S] clusters and the g approximately 2.04 signal of a protein-bound dinitrosyl-iron-dithiol complex in the d7 state. In addition, in the reaction of cytosolic aconitase, the transient formation of a thiyl radical, g parallel = 2.11 and g perpendicular = 2.03, is observed. Disassembly of the [3Fe-4S] clusters of the inactive forms of the enzymes upon the anaerobic addition of NO is also accompanied by the formation of the g approximately 2.04 species and in the case of mitochondrial aconitase, a transient signal at g approximately 2. 032 appeared. This signal is tentatively assigned to the d9 form of an iron-nitrosyl-histidyl complex of the mitochondrial protein. Inactivation of the [4Fe-4S] forms of both aconitases by either superoxide anion or peroxynitrite produces the g = 2.02 [3Fe-4S] proteins.

摘要

细胞研究表明,一些铁硫蛋白,尤其是乌头酸酶,是一氧化氮的作用靶点。具体而言,一氧化氮参与了细胞内的一个过程,即含有[4Fe-4S]簇的活性胞质乌头酸酶转化为其脱辅基形式,该脱辅基形式作为一种铁调节蛋白发挥作用。我们通过跟踪酶活性并观察原始反应物未显示的电子顺磁共振(EPR)信号的形成,对一氧化氮与纯化形式的线粒体和胞质乌头酸酶的反应进行了体外研究。在厌氧条件下,两种酶同工型都可被一氧化氮溶液或产生一氧化氮的硝普钠灭活。这种灭活在有或没有底物的情况下都会发生,同时会出现[3Fe-4S]簇的g = 2.02信号以及处于d7状态的蛋白质结合二亚硝基铁二硫醇配合物的g约为2.04信号。此外,在胞质乌头酸酶的反应中,观察到了一个硫自由基的瞬时形成,其g平行 = 2.11,g垂直 = 2.03。在厌氧条件下向无活性形式的酶中添加一氧化氮后,[3Fe-4S]簇的拆解也伴随着g约为2.04物种的形成,对于线粒体乌头酸酶,还出现了一个g约为2.032的瞬时信号。该信号初步被认为是线粒体蛋白的铁亚硝基组氨酸配合物的d9形式。超氧阴离子或过氧亚硝酸盐使两种乌头酸酶的[4Fe-4S]形式失活,都会产生g = 2.02的[3Fe-4S]蛋白。

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