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编码大肠杆菌乙酰辅酶A羧化酶两个羧基转移酶亚基的基因。

The genes encoding the two carboxyltransferase subunits of Escherichia coli acetyl-CoA carboxylase.

作者信息

Li S J, Cronan J E

机构信息

Department of Microbiology, University of Illinois, Urbana-Champaign 61801.

出版信息

J Biol Chem. 1992 Aug 25;267(24):16841-7.

PMID:1355089
Abstract

We report characterization of the component proteins and molecular cloning of the genes encoding the two subunits of the carboxyltransferase component of the Escherichia coli acetyl-CoA carboxylase. Peptide mapping of the purified enzyme component indicates that the carboxyltransferase component is a complex of two nonidentical subunits, a 35-kDa alpha subunit and a 33-kDa beta subunit. The alpha subunit gene encodes a protein of 319 residues and is located immediately downstream of the polC gene (min 4.3 of the E. coli genetic map). The deduced amino acid composition, molecular mass, and amino acid sequence match those determined for the purified alpha subunit. Six sequenced internal peptides also match the deduced sequence. The amino-terminal sequence of the beta subunit was found within a previously identified open reading frame of unknown function called dedB and usg (min 50 of the E. coli genetic map) which encodes a protein of 304 residues. Comparative peptide mapping also indicates that the dedB/usg gene encodes the beta subunit. Moreover, the deduced molecular mass and amino acid composition of the dedB/usg-encoded protein closely match those determined for the beta subunit. The deduced amino acid sequences of alpha and beta subunits show marked sequence similarities to the COOH-terminal half and the NH2-terminal halves, respectively, of the rat propionyl-CoA carboxylase, a biotin-dependent carboxylase that catalyzes a similar carboxyltransferase reaction reaction. Several conserved regions which may function as CoA-binding sites are noted.

摘要

我们报道了大肠杆菌乙酰辅酶A羧化酶羧基转移酶组分的组成蛋白特性以及编码该组分两个亚基的基因的分子克隆。对纯化的酶组分进行肽图谱分析表明,羧基转移酶组分是由两个不同亚基组成的复合物,一个35 kDa的α亚基和一个33 kDa的β亚基。α亚基基因编码一个含319个残基的蛋白质,位于polC基因(大肠杆菌遗传图谱的4.3分钟处)的紧邻下游。推导的氨基酸组成、分子量和氨基酸序列与纯化的α亚基所确定的一致。六个测序的内部肽段也与推导序列匹配。在先前鉴定的一个功能未知的开放阅读框dedB和usg(大肠杆菌遗传图谱的50分钟处)中发现了β亚基的氨基末端序列,该阅读框编码一个含304个残基的蛋白质。比较肽图谱分析也表明dedB/usg基因编码β亚基。此外,dedB/usg编码蛋白的推导分子量和氨基酸组成与β亚基所确定的紧密匹配。α亚基和β亚基的推导氨基酸序列分别与大鼠丙酰辅酶A羧化酶的羧基末端一半和氨基末端一半有显著的序列相似性,大鼠丙酰辅酶A羧化酶是一种生物素依赖性羧化酶,催化类似的羧基转移酶反应。注意到几个可能作为辅酶A结合位点的保守区域。

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