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在大肠杆菌crp基因3'侧翼序列中产生缺失,这些缺失可诱导环磷酸腺苷抑制功能。

Generation of deletions in the 3'-flanking sequences of the Escherichia coli crp gene that induce cyclic AMP suppressor functions.

作者信息

Barton J W, Melton T

出版信息

J Bacteriol. 1987 Feb;169(2):654-9. doi: 10.1128/jb.169.2.654-659.1987.

Abstract

The crp structural gene and its 3'-flanking sequences were subcloned into M13mp8, and in vitro deletions were constructed in both the 5' and 3' ends of the gene by using Bal 31 nuclease. Deletions ranged in size from 24 to 250 base pairs at the 5' end of crp. Sixteen deletions generated at the 3' end of the gene ranged in size from 133 to 675 base pairs. The majority of deletions extended into the crp structural gene. Another class of deletions, i.e., delta crp-4, delta crp-17, and delta crp-2, had endpoints extending in the 3'-flanking sequences external to the crp structural gene. Deletions were subcloned into pBR322 and transformed into the Escherichia coli cya crp deletion strain NCR438. Transformants containing plasmid pBM4 with the delta crp4 mutation, a deletion of 133 base pairs, were cyclic AMP independent. Strain NCR440 harboring this plasmid expressed beta-galactosidase and threonine dehydratase activities and fermented lactose, ribose, arabinose, and xylose in the absence of exogenous cyclic AMP. The delta crp-4 mutation also caused strain NCR440 to be hypersensitive to exogenous cyclic AMP. The cylic AMP receptor protein expressed in maxicells from pBM4 carrying the delta crp-4 mutation comigrated with the wild-type protein on electrophoretic gels. The delta crp-4 mutation demonstrates that sequences distal to the crp structural gene can mediate cyclic AMP suppressor functions.

摘要

将crp结构基因及其3'侧翼序列亚克隆到M13mp8中,利用Bal 31核酸酶在基因的5'和3'末端构建体外缺失。crp 5'端缺失的大小范围为24至250个碱基对。在基因3'端产生的16个缺失大小范围为133至675个碱基对。大多数缺失延伸到crp结构基因中。另一类缺失,即δcrp - 4、δcrp - 17和δcrp - 2,其端点延伸到crp结构基因外部的3'侧翼序列中。将缺失片段亚克隆到pBR322中,并转化到大肠杆菌cya crp缺失菌株NCR438中。含有带有δcrp4突变(缺失133个碱基对)的质粒pBM4的转化体不依赖于环磷酸腺苷。携带该质粒的菌株NCR440在没有外源环磷酸腺苷的情况下表达β-半乳糖苷酶和苏氨酸脱水酶活性,并发酵乳糖、核糖、阿拉伯糖和木糖。δcrp - 4突变还导致菌株NCR440对外源环磷酸腺苷高度敏感。在携带δcrp - 4突变的pBM4的大细胞中表达的环磷酸腺苷受体蛋白在电泳凝胶上与野生型蛋白共迁移。δcrp - 4突变表明crp结构基因远端的序列可以介导环磷酸腺苷抑制功能。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5389/211828/0465b33e6c32/jbacter00192-0224-a.jpg

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