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大肠杆菌K-12中外膜蛋白合成的调控:ompC缺失影响OmpF蛋白的表达。

Regulation of outer membrane protein synthesis in Escherichia coli K-12: deletion of ompC affects expression of the OmpF protein.

作者信息

Schnaitman C A, McDonald G A

出版信息

J Bacteriol. 1984 Aug;159(2):555-63. doi: 10.1128/jb.159.2.555-563.1984.

Abstract

A chromosomal deletion beginning at a Tn10 located ca. 8 kilobases upstream from the ompC structural gene and extending through the 2.6-kilobase HindIII fragment carrying the ompC was isolated. The 2.6-kilobase ompC fragment was cloned into lambda 540 to obtain phage lambda 540C1. When the deletion mutant was lysogenized with lambda 540C1, the resulting strain produced normal levels of OmpC protein, and expression of this protein was regulated by osmolarity, carbon source, and the lc gene of phage PA-2, indicating that the cloned fragment contained all of the information required for regulated expression of ompC. The strain carrying the deletion was partially constitutive for expression of OmpF protein, whereas the lambda 540C1 lysogen of this strain and other strains with mutations in ompC repressed OmpF synthesis under conditions which lead to high-level expression of OmpC protein. Strains which are diploid or triploid for ompC show strong inhibition of synthesis of OmpF protein. We conclude that a regulatory element located upstream from the ompC coding sequence inhibits translation of OmpF protein under conditions which favor OmpC expression. Since ompF is known to repress transcription of ompC, we propose that these two genes constitute a closed regulatory loop which acts to amplify regulatory signals which control expression of these proteins.

摘要

分离出一种染色体缺失突变体,其缺失起始于位于ompC结构基因上游约8千碱基处的Tn10,并延伸至携带ompC的2.6千碱基HindIII片段。将2.6千碱基的ompC片段克隆到λ540中,得到噬菌体λ540C1。当用λ540C1使缺失突变体溶源化时,所得菌株产生正常水平的OmpC蛋白,并且该蛋白的表达受渗透压、碳源和噬菌体PA - 2的lc基因调控,这表明克隆片段包含ompC调控表达所需的所有信息。携带缺失的菌株在OmpF蛋白表达上部分组成型,而该菌株的λ540C1溶源菌以及其他ompC有突变的菌株在导致OmpC蛋白高水平表达的条件下抑制OmpF的合成。对于ompC是二倍体或三倍体的菌株显示出对OmpF蛋白合成的强烈抑制。我们得出结论,位于ompC编码序列上游的一个调控元件在有利于OmpC表达的条件下抑制OmpF蛋白的翻译。由于已知ompF抑制ompC的转录,我们提出这两个基因构成一个封闭的调控环,其作用是放大控制这些蛋白质表达的调控信号。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a24e/215679/92cb9d5c081c/jbacter00231-0133-a.jpg

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