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编码大肠杆菌甘氨酸裂解系统的gcv操纵子的克隆与核苷酸序列

Cloning and nucleotide sequence of the gcv operon encoding the Escherichia coli glycine-cleavage system.

作者信息

Okamura-Ikeda K, Ohmura Y, Fujiwara K, Motokawa Y

机构信息

Institute for Enzyme Research, University of Tokushima, Japan.

出版信息

Eur J Biochem. 1993 Sep 1;216(2):539-48. doi: 10.1111/j.1432-1033.1993.tb18172.x.

DOI:10.1111/j.1432-1033.1993.tb18172.x
PMID:8375392
Abstract

P-protein, H-protein and T-protein of the glycine cleavage system have been purified from Escherichia coli. Their N-terminal amino acid sequences were determined, and a set of oligonucleotide probes was designed for gene cloning. The nucleotide sequence of a fragment of DNA around the 62-min region of the E. coli chromosome, containing genes for the components of the glycine-cleavage system has been determined. The sequence includes three structural genes encoding T-protein (363 amino acids, 40013 Da), H-protein (128 amino acids, 13679 Da) and P-protein (956 amino acids, 104240 Da). These genes are named gcvT, gcvH and gcvP, respectively. They are organized in the above-mentioned order on the same strand of DNA with short intercistronic sequences. The presence of a potential promoter preceding gcvT and a typical rho-independent terminator sequence following gcvP indicated that the three genes constitute a single operon. Each component of the E. coli glycine-cleavage system exhibits considerable amino acid sequence similarity with the animal and plant counterparts. When the plasmid containing the gcv operon was transfected in E. coli cells, the gene products of gcvT, gcvH and gcvP were overexpressed under the direction of the promoter of the gcv operon. However, bacteria harboring the plasmid that contained the gcv operon without the promoter region and the 5' terminal portion of gcvT failed to overexpress any of the three components.

摘要

甘氨酸裂解系统的P蛋白、H蛋白和T蛋白已从大肠杆菌中纯化出来。测定了它们的N端氨基酸序列,并设计了一组寡核苷酸探针用于基因克隆。已确定大肠杆菌染色体62分钟区域附近一段DNA片段的核苷酸序列,该片段包含甘氨酸裂解系统各组分的基因。该序列包括三个结构基因,分别编码T蛋白(363个氨基酸,40013道尔顿)、H蛋白(128个氨基酸,13679道尔顿)和P蛋白(956个氨基酸,104240道尔顿)。这些基因分别命名为gcvT、gcvH和gcvP。它们以上述顺序排列在DNA的同一条链上,基因间序列较短。gcvT之前存在一个潜在的启动子,gcvP之后存在一个典型的不依赖ρ因子的终止子序列,这表明这三个基因构成一个单一的操纵子。大肠杆菌甘氨酸裂解系统的每个组分与动植物相应组分都表现出相当程度的氨基酸序列相似性。当将含有gcv操纵子的质粒转染到大肠杆菌细胞中时,gcvT、gcvH和gcvP的基因产物在gcv操纵子启动子的指导下过表达。然而,携带不含启动子区域和gcvT 5'末端部分的gcv操纵子的质粒的细菌未能过表达这三种组分中的任何一种。

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