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通过将丙氨酸95定点突变为甘氨酸,将L-乳酸氧化酶转化为长链α-羟基酸氧化酶。

Conversion of L-lactate oxidase to a long chain alpha-hydroxyacid oxidase by site-directed mutagenesis of alanine 95 to glycine.

作者信息

Yorita K, Aki K, Ohkuma-Soyejima T, Kokubo T, Misaki H, Massey V

机构信息

Institute for Enzyme Research, University of Tokushima, Tokushima 770, Japan.

出版信息

J Biol Chem. 1996 Nov 8;271(45):28300-5. doi: 10.1074/jbc.271.45.28300.

Abstract

A mutant form of L-lactate oxidase (LOX) from Aerococcus viridans in which alanine 95 was replaced by glycine was constructed as a mimic of L-lactate monooxygenase but proved instead to be a mimic of the long chain alpha-hydroxyacid oxidase from rat kidney. A95G-LOX keeps oxidase activity with L-lactate at the same level as wild type LOX but has much enhanced oxidase activity with longer chain L-alpha-hydroxyacids, alpha-hydroxy-n-butyric acid, alpha-hydroxy-n-valeric acid, etc., and also the aromatic alpha-hydroxyacid, L-mandelic acid. Kinetic analysis of the activity with these substrates indicates that the reduction of the enzyme bound flavin by substrates is the rate-limiting step in A95G-LOX. The affinity of pyruvate for the reduced enzyme is increased, and sulfite binding to the oxidized enzyme is weaker in A95G-LOX than in native enzyme. Wild type LOX stabilizes both the neutral and anionic flavin semiquinones with a pKa of 6.1, but A95G LOX stabilizes only the anionic semiquinone form. These results strongly suggest that the environment around the N5-C4a region of the flavin isoalloxazine ring is changed by this mutation.

摘要

构建了绿色气球菌L-乳酸氧化酶(LOX)的一种突变形式,其中第95位丙氨酸被甘氨酸取代,作为L-乳酸单加氧酶的模拟物,但结果证明它是大鼠肾脏中长链α-羟基酸氧化酶的模拟物。A95G-LOX对L-乳酸的氧化酶活性与野生型LOX处于同一水平,但对更长链的L-α-羟基酸、α-羟基正丁酸、α-羟基正戊酸等以及芳香族α-羟基酸L-扁桃酸的氧化酶活性有很大增强。对这些底物活性的动力学分析表明,底物对酶结合黄素的还原是A95G-LOX中的限速步骤。丙酮酸对还原酶的亲和力增加,并且在A95G-LOX中,亚硫酸盐与氧化酶的结合比天然酶中更弱。野生型LOX稳定pKa为6.1的中性和阴离子型黄素半醌,但A95G LOX仅稳定阴离子型半醌形式。这些结果强烈表明,黄素异咯嗪环N5-C4a区域周围的环境因该突变而改变。

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