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枯草芽孢杆菌克隆的gyrA和gyrB基因的遗传与物理组织

Genetic and physical organization of the cloned gyrA and gyrB genes of Bacillus subtilis.

作者信息

Lampe M F, Bott K F

出版信息

J Bacteriol. 1985 Apr;162(1):78-84. doi: 10.1128/jb.162.1.78-84.1985.

Abstract

An 8-kilobase fragment already known to contain the gyrA gene of Bacillus subtilis was shown to encode the gyrB gene as well. Plasmids containing this fragment can rescue both B. subtilis gyrA and gyrB mutants and complement Escherichia coli gyrA mutants. Deletion analysis has indicated the gene locations on the cloned fragment. Under low-stringency conditions the cloned E. coli gyrA and gyrB genes each hybridized to the appropriate subfragments, confirming the assignment of the gene locations on the cloned DNA. In E. coli maxicells, proteins of 67,000 (gyrA) and 77,000 (gyrB) Mr were synthesized. Analysis of proteins encoded by various subfragments indicated the direction of transcription. Although the gyrA and gyrB genes are located adjacent to each other on the chromosome, they may be transcribed independently since expression of gyrA protein is not dependent upon the gyrB gene in maxicells.

摘要

一个已知包含枯草芽孢杆菌gyrA基因的8千碱基片段也被证明编码gyrB基因。含有该片段的质粒可以拯救枯草芽孢杆菌gyrA和gyrB突变体,并补充大肠杆菌gyrA突变体。缺失分析已表明克隆片段上的基因位置。在低严格条件下,克隆的大肠杆菌gyrA和gyrB基因各自与适当的亚片段杂交,证实了克隆DNA上基因位置的确定。在大肠杆菌的大细胞中,合成了分子量为67,000(gyrA)和77,000(gyrB)的蛋白质。对各种亚片段编码的蛋白质分析表明了转录方向。尽管gyrA和gyrB基因在染色体上彼此相邻,但它们可能独立转录,因为在大细胞中gyrA蛋白的表达不依赖于gyrB基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/587d/218956/cf47cdcdd25f/jbacter00221-0090-a.jpg

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