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Citrate synthase activity in Escherichia coli harbouring hybrid plasmids containing the gltA gene.

作者信息

Bloxham D P, Herbert C J, Ner S S, Drabble W T

出版信息

J Gen Microbiol. 1983 Jun;129(6):1889-97. doi: 10.1099/00221287-129-6-1889.

DOI:10.1099/00221287-129-6-1889
PMID:6355385
Abstract

A hybrid plasmid, pDB2, was constructed by ligating a 3.24 kb EcoRI/HindIII fragment of the Escherichia coli chromosome into pBR322. This was used to transform a gltA mutant which was devoid of citrate synthase activity. The resultant strain expressed very high citrate synthase activity and this enabled a simplified purification of the homogeneous enzyme in high yield. The subunit Mr was estimated as 47000-49000 by SDS gel electrophoresis, which closely resembles the eukaryotic form of the enzyme. Evidence for some conservation of sequence between the two proteins was revealed in the acid cleavage pattern at aspartyl-prolyl residues. In addition to coding for the structural gene for citrate synthase, the 3.24 kb EcoRI/HindIII fragment also retained the genetic structure necessary for control of enzyme synthesis since the expression of enzyme activity in the strain harbouring pDB2 was still subject to glucose repression.

摘要

相似文献

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Aspartase-hyperproducing mutants of Escherichia coli B.大肠杆菌B的天冬氨酸酶高产突变体
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The use of bacteriophage M13 carrying defined fragments of the Escherichia coli gltA gene to determine the location and structure of the citrate synthase promoter region.
利用携带大肠杆菌gltA基因特定片段的噬菌体M13来确定柠檬酸合酶启动子区域的位置和结构。
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