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可自动催化修饰其辅基血红素基团的辣根过氧化物酶突变体:对哺乳动物过氧化物酶血红素 - 蛋白质共价键的见解。

Horseradish peroxidase mutants that autocatalytically modify their prosthetic heme group: insights into mammalian peroxidase heme-protein covalent bonds.

作者信息

Colas Christophe, De Montellano Paul R Ortiz

机构信息

Department of Pharmaceutical Chemistry, University of California, San Francisco, California 94143-2280, USA.

出版信息

J Biol Chem. 2004 Jun 4;279(23):24131-40. doi: 10.1074/jbc.M401687200. Epub 2004 Mar 23.

DOI:10.1074/jbc.M401687200
PMID:15039425
Abstract

The mammalian peroxidases, including myeloperoxidase and lactoperoxidase, bind their prosthetic heme covalently through ester bonds to two of the heme methyl groups. These bonds are autocatalytically formed. No other peroxidase is known to form such bonds. To determine whether features other than an appropriately placed carboxylic acid residue are important for covalent heme binding, we have introduced aspartate and/or glutamic acid residues into horseradish peroxidase, a plant enzyme that exhibits essentially no sequence identity with the mammalian peroxidases. Based on superposition of the horseradish peroxidase and myeloperoxidase structures, the mutated residues were Leu(37), Phe(41), Gly(69), and Ser(73). The F41E mutant was isolated with no covalently bound heme, but the heme was completely covalently bound upon incubation with H(2)O(2). As predicted, the modified heme released from the protein was 3-hydroxymethylheme. The S73E mutant did not covalently bind its heme but oxidized it to the 8-hydroxymethyl derivative. The hydroxyl group in this modified heme derived from the medium. The other mutations gave unstable proteins. The rate of compound I formation for the F41E mutant was 100 times faster after covalent bond formation, but the reduction of compound I to compound II was similar with and without the covalent bond. The results clearly establish that an appropriately situated carboxylic acid group is sufficient for covalent heme attachment, strengthen the proposed mechanism, and suggest that covalent heme attachment in the mammalian peroxidases relates to peroxidase biology or stability rather than to intrinsic catalytic properties.

摘要

包括髓过氧化物酶和乳过氧化物酶在内的哺乳动物过氧化物酶,通过酯键将其辅基血红素与血红素的两个甲基共价结合。这些键是自动催化形成的。已知没有其他过氧化物酶会形成这样的键。为了确定除了位置合适的羧酸残基之外,其他特征对于血红素的共价结合是否重要,我们已将天冬氨酸和/或谷氨酸残基引入辣根过氧化物酶中,这种植物酶与哺乳动物过氧化物酶基本上没有序列同源性。基于辣根过氧化物酶和髓过氧化物酶结构的叠加,突变的残基为Leu(37)、Phe(41)、Gly(69)和Ser(73)。F41E突变体分离出来时没有共价结合的血红素,但与H₂O₂孵育后血红素完全共价结合。正如所预测的,从蛋白质中释放出来的修饰血红素是3 - 羟甲基血红素。S73E突变体没有共价结合其血红素,但将其氧化为8 - 羟甲基衍生物。这种修饰血红素中的羟基来源于培养基。其他突变产生了不稳定的蛋白质。共价键形成后,F41E突变体形成化合物I的速率快100倍,但化合物I还原为化合物II的过程在有或没有共价键的情况下相似。结果清楚地表明,一个位置合适的羧酸基团足以实现血红素的共价附着,强化了所提出的机制,并表明哺乳动物过氧化物酶中血红素的共价附着与过氧化物酶生物学或稳定性有关,而不是与内在催化特性有关。

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