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来自大肠杆菌的两种延胡索酸酶的纯化与特性分析

Purification and characterization of two types of fumarase from Escherichia coli.

作者信息

Ueda Y, Yumoto N, Tokushige M, Fukui K, Ohya-Nishiguchi H

机构信息

Department of Chemistry, Faculty of Science, Kyoto University.

出版信息

J Biochem. 1991 May;109(5):728-33. doi: 10.1093/oxfordjournals.jbchem.a123448.

Abstract

Two distinct types of fumarase were purified to homogeneity from aerobically grown Escherichia coli W cells. The amino acid sequences of their NH2-terminals suggest that the two enzymes are the products of the fumA gene (FUMA) and fumC gene (FUMC), respectively. FUMA was separated from FUMC by chromatography on a Q-Sepharose column, and was further purified to homogeneity on Alkyl-Superose, Mono Q, and Superose 12 columns. FUMA is a dimer composed of identical subunits (Mr = 60,000). Although the activity of FUMA rapidly decreased during storage, reactivation was attained by anaerobic incubation with Fe2+ and thiols. Studies on the inactivation and reactivation of FUMA suggested that oxidation and the concomitant release of iron inactivated the enzyme in a reversible manner. While the inactivated FUMA was EPR-detectable, through a signal with g perpendicular = 2.02 and g = 2.00, the active enzyme was EPR-silent. These results suggested FUMA is a member of the 4Fe-4S hydratases represented by aconitase. After the separation of FUMC from FUMA, purification of the former enzyme was accomplished by chromatography on Phenyl-Superose and Matrex Gel Red A columns. FUMC was stable, Fe-independent and quite similar to mammalian fumarases in enzymatic properties.

摘要

从需氧生长的大肠杆菌W细胞中纯化出两种不同类型的延胡索酸酶,使其达到同质状态。它们氨基末端的氨基酸序列表明,这两种酶分别是fumA基因(FUMA)和fumC基因(FUMC)的产物。通过在Q-Sepharose柱上进行层析将FUMA与FUMC分离,并在烷基-超级琼脂糖、单Q和超级琼脂糖12柱上进一步纯化至同质状态。FUMA是由相同亚基组成的二聚体(Mr = 60,000)。尽管FUMA的活性在储存过程中迅速下降,但通过与Fe2+和硫醇进行厌氧孵育可实现再激活。对FUMA失活和再激活的研究表明,氧化以及随之而来的铁释放以可逆方式使该酶失活。虽然失活的FUMA可通过g垂直 = 2.02和g = 2.00的信号进行电子顺磁共振(EPR)检测,但活性酶在EPR检测中无信号。这些结果表明FUMA是由乌头酸酶代表的4Fe-4S水合酶家族的成员。从FUMA中分离出FUMC后,通过在苯基-超级琼脂糖和Matrex Gel Red A柱上进行层析完成了前一种酶的纯化。FUMC稳定,不依赖铁,并且在酶学性质上与哺乳动物延胡索酸酶非常相似。

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