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大肠杆菌的glc基因座:编码乙醇酸氧化酶亚基和glc调节蛋白的基因的特征

glc locus of Escherichia coli: characterization of genes encoding the subunits of glycolate oxidase and the glc regulator protein.

作者信息

Pellicer M T, Badía J, Aguilar J, Baldomà L

机构信息

Department of Biochemistry, Faculty of Pharmacy, University of Barcelona, Spain.

出版信息

J Bacteriol. 1996 Apr;178(7):2051-9. doi: 10.1128/jb.178.7.2051-2059.1996.

Abstract

The locus glc (min 64.5), associated with the glycolate utilization trait in Escherichia coli, is known to contain glcB, encoding malate synthase G, and the gene(s) needed for glycolate oxidase activity. Subcloning, sequencing, insertion mutagenesis, and expression studies showed five additional genes: glcC and in the other direction glcD, glcE, glcF, and glcG followed by glcB. The gene glcC may encode the glc regulator protein. Consistently a chloramphenicol acetyltransferase insertion mutation abolished both glycolate oxidase and malate synthase G activities. The proteins encoded from glcD and glcE displayed similarity to several flavoenzymes, the one from glcF was found to be similar to iron-sulfur proteins, and that from glcG had no significant similarity to any group of proteins. The insertional mutation by a chloramphenicol acetyltransferase cassette in either glcD, glcE, or glcF abolished glycolate oxidase activity, indicating that presumably these proteins are subunits of this enzyme. No effect on glycolate metabolism was detected by insertional mutation in glcG. Northern (RNA) blot experiments showed constitutive expression of glcC but induced expression for the structural genes and provided no evidence for a single polycistronic transcript.

摘要

与大肠杆菌中乙醇酸利用性状相关的基因座glc(最小64.5),已知包含编码苹果酸合酶G的glcB以及乙醇酸氧化酶活性所需的基因。亚克隆、测序、插入诱变和表达研究显示还有五个基因:glcC,以及在另一个方向上的glcD、glcE、glcF和glcG,其后是glcB。基因glcC可能编码glc调节蛋白。一致地,氯霉素乙酰转移酶插入突变消除了乙醇酸氧化酶和苹果酸合酶G的活性。glcD和glcE编码的蛋白质与几种黄素酶具有相似性,glcF编码的蛋白质与铁硫蛋白相似,而glcG编码的蛋白质与任何蛋白质组均无明显相似性。氯霉素乙酰转移酶盒在glcD、glcE或glcF中的插入突变消除了乙醇酸氧化酶活性,这表明大概这些蛋白质是该酶的亚基。glcG中的插入突变未检测到对乙醇酸代谢的影响。Northern(RNA)印迹实验显示glcC组成型表达,但结构基因是诱导型表达,并且没有证据表明存在单一的多顺反子转录本。

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