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大肠杆菌延胡索酸还原酶膜锚定多肽的鉴定

Identification of membrane anchor polypeptides of Escherichia coli fumarate reductase.

作者信息

Lemire B D, Robinson J J, Weiner J H

出版信息

J Bacteriol. 1982 Dec;152(3):1126-31. doi: 10.1128/jb.152.3.1126-1131.1982.

Abstract

Fumarate reductase of Escherichia coli has been shown to be a membrane-bound enzyme composed of a 69,000-dalton catalytic-flavin-containing subunit and a 27,000-dalton nonheme-iron-containing subunit. Using gene cloning and amplification techniques, we have observed two additional polypeptides encoded by the frd operon, with apparent molecular weights of 15,000 and 14,000, which are expressed when E. coli is grown anaerobically on glycerol plus fumarate. Expression of these two small polypeptides is necessary for the two large subunits to associate with the membrane. The four subunits remain associated in Triton X-100 extracts of the membrane, and a holoenzyme form of fumarate reductase containing one copy of each of the four polypeptides has been isolated. Unlike the well-characterized two-subunit form, the holoenzyme is not dependent on anions for activity and is not labile at alkaline pH. In these respects, it more closely resembles the membrane-bound activity.

摘要

大肠杆菌的延胡索酸还原酶已被证明是一种膜结合酶,由一个69,000道尔顿含催化黄素的亚基和一个27,000道尔顿含非血红素铁的亚基组成。利用基因克隆和扩增技术,我们观察到frd操纵子编码的另外两种多肽,表观分子量分别为15,000和14,000,当大肠杆菌在甘油加延胡索酸上厌氧生长时表达。这两种小多肽的表达是两个大亚基与膜结合所必需的。这四个亚基在膜的Triton X-100提取物中保持结合状态,并且已经分离出一种含有四种多肽各一个拷贝的延胡索酸还原酶全酶形式。与特征明确的二亚基形式不同,全酶的活性不依赖于阴离子,在碱性pH下也不稳定。在这些方面,它更类似于膜结合活性。

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