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碳酸氢根辅因子调节大肠杆菌menaquinone 生物合成中的 1,4-二羟基-2-萘酰基辅酶 A 合酶。

A bicarbonate cofactor modulates 1,4-dihydroxy-2-naphthoyl-coenzyme a synthase in menaquinone biosynthesis of Escherichia coli.

机构信息

Department of Chemistry, State Key Laboratory of Molecular Neuroscience, The Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, Hong Kong, China.

出版信息

J Biol Chem. 2010 Sep 24;285(39):30159-69. doi: 10.1074/jbc.M110.147702. Epub 2010 Jul 19.

Abstract

1,4-Dihydroxy-2-naphthoyl coenzyme A (DHNA-CoA) synthase is a typical crotonase-fold protein catalyzing an intramolecular Claisen condensation in the menaquinone biosynthetic pathway. We have characterized this enzyme from Escherichia coli and found that it is activated by bicarbonate in a concentration-dependent manner. The bicarbonate binding site has been identified in the crystal structure of a virtually identical ortholog (96.8% sequence identity) from Salmonella typhimurium through comparison with a bicarbonate-insensitive orthologue. Kinetic properties of the enzyme and its site-directed mutants of the bicarbonate binding site indicate that the exogenous bicarbonate anion is essential to the enzyme activity. With this essential catalytic role, the simple bicarbonate anion is an enzyme cofactor, which is usually a small organic molecule derived from vitamins, a metal ion, or a metal-containing polyatomic anionic complex. This finding leads to classification of the DHNA-CoA synthases into two evolutionarily conserved subfamilies: type I enzymes that are bicarbonate-dependent and contain a conserved glycine at the bicarbonate binding site; and type II enzymes that are bicarbonate-independent and contain a conserved aspartate at the position similar to the enzyme-bound bicarbonate. In addition, the unique location of the enzyme-bound bicarbonate allows it to be proposed as a catalytic base responsible for abstraction of the α-proton of the thioester substrate in the enzymatic reaction, suggesting a unified catalytic mechanism for all DHNA-CoA synthases.

摘要

1,4-二羟基-2-萘酰辅酶 A(DHNA-CoA)合酶是一种典型的克罗顿酶折叠蛋白,催化类异戊二烯醌生物合成途径中的分子内克莱森缩合反应。我们已经从大肠杆菌中鉴定出这种酶,并发现它在浓度依赖性方式下被碳酸氢盐激活。通过与碳酸氢盐不敏感的同源物进行比较,在来自鼠伤寒沙门氏菌的几乎相同的同源物的晶体结构中已经鉴定出碳酸氢盐结合位点。酶及其碳酸氢盐结合位点的定点突变体的动力学特性表明,外源性碳酸氢盐阴离子对于酶活性是必需的。由于这种必需的催化作用,简单的碳酸氢盐阴离子是一种酶辅因子,通常是来自维生素、金属离子或含金属的多原子阴离子配合物的小分子有机分子。这一发现将 DHNA-CoA 合酶分为两个进化上保守的亚家族:依赖碳酸氢盐的 I 型酶,其碳酸氢盐结合位点含有保守的甘氨酸;以及独立于碳酸氢盐的 II 型酶,其在类似于酶结合的碳酸氢盐的位置含有保守的天冬氨酸。此外,酶结合的碳酸氢盐的独特位置使其可以被提议作为负责在酶反应中提取硫酯底物的α-质子的催化碱,这表明所有 DHNA-CoA 合酶都具有统一的催化机制。

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