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大肠杆菌环丙烷脂肪酸合酶基因的克隆与操作:酶过量表达的生理学方面

Cloning and manipulation of the Escherichia coli cyclopropane fatty acid synthase gene: physiological aspects of enzyme overproduction.

作者信息

Grogan D W, Cronan J E

出版信息

J Bacteriol. 1984 Apr;158(1):286-95. doi: 10.1128/jb.158.1.286-295.1984.

Abstract

Like many other eubacteria, cultures of Escherichia coli accumulate cyclopropane fatty acids (CFAs) at a well-defined stage of growth, due to the action of the cytoplasmic enzyme CFA synthase. We report the isolation of the putative structural gene, cfa, for this enzyme on an E. coli-ColE1 chimeric plasmid by the use of an autoradiographic colony screening technique. When introduced into a variety of E. coli strains, this plasmid, pLC18-11, induced corresponding increases in CFA content and CFA synthase activity. Subsequent manipulation of the cfa locus, facilitated by the insertion of pLC18-11 into a bacteriophage lambda vector, allowed genetic and physiological studies of CFA synthase in E. coli. Overproduction of this enzyme via multicopy cfa plasmids caused abnormally high levels of CFA in membrane phospholipid but no discernable growth perturbation. Infection with phage lambda derivatives bearing cfa caused transient overproduction of the enzyme, although pL-mediated expression of cfa could not be demonstrated in plasmids derived from such phages. CFA synthase specific activities could be raised to very high levels by using cfa runaway-replication plasmids. A variety of physiological factors were found to modulate the levels of CFA synthase in normal and gene-amplified cultures. These studies argue against several possible mechanisms for the temporal regulation of CFA formation.

摘要

与许多其他真细菌一样,由于细胞质酶环丙烷脂肪酸合酶的作用,大肠杆菌培养物在生长的特定阶段积累环丙烷脂肪酸(CFA)。我们报告了通过使用放射自显影片落筛选技术,在大肠杆菌 - ColE1嵌合质粒上分离出该酶的推定结构基因cfa。当将该质粒pLC18 - 11导入多种大肠杆菌菌株时,会相应增加CFA含量和CFA合酶活性。随后,通过将pLC18 - 11插入噬菌体λ载体,便于对cfa基因座进行操作,从而对大肠杆菌中的CFA合酶进行遗传和生理学研究。通过多拷贝cfa质粒过量生产这种酶会导致膜磷脂中CFA水平异常升高,但未观察到明显的生长干扰。用携带cfa的噬菌体λ衍生物感染会导致该酶的短暂过量生产,尽管在由此类噬菌体衍生的质粒中无法证明cfa的pL介导表达。通过使用cfa失控复制质粒,CFA合酶的比活性可以提高到非常高的水平。发现多种生理因素可调节正常培养物和基因扩增培养物中CFA合酶的水平。这些研究反对CFA形成的时间调节的几种可能机制。

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