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从无镍前体形式体外生成活性[NiFe]氢化酶。

Generation of active [NiFe] hydrogenase in vitro from a nickel-free precursor form.

作者信息

Maier T, Böck A

机构信息

Lehrstuhl für Mikrobiologie, Universität München, Germany.

出版信息

Biochemistry. 1996 Aug 6;35(31):10089-93. doi: 10.1021/bi960567l.

Abstract

The maturation process of [NiFe] hydrogenases includes formation of the nickel metallocenter, proteolytic processing of the large subunit, and assembly with the other hydrogenase subunit(s). An in vitro system for the maturation of the large subunit (HycE) of hydrogenase 3 of Escherichia coli leading to an active enzyme was established. The system is based on extracts of an E. coli mutant lacking the nickel-specific transport system (nik). HycE was present in these extracts in the C-terminally extended precursor form devoid of nickel. Addition of nickel led to nickel incorporation and proteolytic processing of HycE. Under anaerobic conditions, hydrogenase 3 activity was subsequently generated. The maximal rate of the processing reaction was reached at a nickel concentration of 400 microM. The accessory proteins known to be involved in the maturation of HycE in vivo, namely HypB, HypC, HypD, HypE, HypF, and the protease HycI, are required for the in vitro reaction, since processing of HycE did not occur in extracts of double mutants affected in the nik system and in one of the accessory genes. Processing of HycE and generation of hydrogenase 3 activity were achieved in extracts of the nik- delta hycI mutant by addition of both nickel and purified HycI protease.

摘要

[NiFe]氢化酶的成熟过程包括镍金属中心的形成、大亚基的蛋白水解加工以及与其他氢化酶亚基的组装。建立了一种体外系统,用于大肠杆菌氢化酶3大亚基(HycE)的成熟,以产生有活性的酶。该系统基于缺乏镍特异性转运系统(nik)的大肠杆菌突变体的提取物。HycE以C末端延伸的前体形式存在于这些提取物中,不含镍。添加镍导致镍掺入和HycE的蛋白水解加工。在厌氧条件下,随后产生了氢化酶3活性。加工反应的最大速率在镍浓度为400微摩尔时达到。已知在体内参与HycE成熟的辅助蛋白,即HypB、HypC、HypD、HypE、HypF和蛋白酶HycI,是体外反应所必需的,因为在nik系统和其中一个辅助基因中受影响的双突变体提取物中未发生HycE的加工。通过添加镍和纯化的HycI蛋白酶,在nik-δhycI突变体的提取物中实现了HycE的加工和氢化酶3活性的产生。

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