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mgpS,一个参与球形红细菌2.4.1中puc和puf操纵子转录调控的复杂调控位点。

mgpS, a complex regulatory locus involved in the transcriptional control of the puc and puf operons in Rhodobacter sphaeroides 2.4.1.

作者信息

Sabaty M, Kaplan S

机构信息

Department of Microbiology and Molecular Genetics, University of Texas Health Science Center at Houston 77225, USA.

出版信息

J Bacteriol. 1996 Jan;178(1):35-45. doi: 10.1128/jb.178.1.35-45.1996.

Abstract

A new method has been developed in order to select mutants showing decreased puc operon transcription in Rhodobacter sphaeroides 2.4.1. A transcriptional fusion of a promoterless fragment derived from the sacB gene, encoding the levansucrase from Bacillus subtilis, to the upstream regulatory region of the puc operon has been constructed. With appropriate levels of exogenous sucrose, survivors of a sucrose killing challenge have been isolated. Subsequent analysis revealed the presence of both cis- and trans-acting "down" mutations in relation to puc operon expression. One of the trans-acting regulatory mutations was chosen for further study. The original mutation showed less than 2% of the level of puc operon transcription compared with the wild type under aerobic conditions and an 86% reduction under dark dimethyl sulfoxide conditions. This mutation can be complemented by a 3.9-kb BamHI DNA fragment derived from a cosmid contained within a genomic cosmid bank. DNA sequence analysis of this fragment revealed the presence of a 2.8-kb open reading frame, designated mgpS, which would encode a 930-amino-acid protein. The N-terminal portion of the putative protein product presents homologies to proteins of the RNA helicase family. Disruption of the chromosomal mgpS resulted in decreased transcription of both puc and puf, while the presence of mgpS in multicopy in the wild type, 2.4.1., increased puc expression by a factor of 2 under aerobic conditions. Structural analysis of the mgpS locus revealed that expression of mgpS was likely to be complex. A smaller protein containing the 472 C-terminal amino acids of MgpS is able to act by itself as an activator of puc transcription and is expressed independently of the large open reading frame in which it is contained.

摘要

为了筛选出球形红细菌2.4.1中puc操纵子转录降低的突变体,人们开发了一种新方法。已构建了一个转录融合体,它将来源于枯草芽孢杆菌果聚糖蔗糖酶的sacB基因的无启动子片段与puc操纵子的上游调控区域融合。在适当水平的外源蔗糖存在下,分离出了蔗糖杀伤挑战的存活者。随后的分析揭示了与puc操纵子表达相关的顺式和反式作用“下调”突变的存在。选择其中一个反式作用调控突变进行进一步研究。与野生型相比,原始突变在有氧条件下puc操纵子转录水平不到2%,在黑暗二甲亚砜条件下降低了86%。该突变可以被来自基因组粘粒文库中一个粘粒的3.9 kb BamHI DNA片段互补。对该片段的DNA序列分析揭示了一个2.8 kb的开放阅读框,命名为mgpS,它编码一个930个氨基酸的蛋白质。推测的蛋白质产物的N端部分与RNA解旋酶家族的蛋白质具有同源性。染色体上mgpS的破坏导致puc和puf的转录减少,而在野生型2.4.1中多拷贝存在mgpS时,在有氧条件下puc表达增加了2倍。mgpS基因座的结构分析表明,mgpS的表达可能很复杂。一个包含MgpS 472个C端氨基酸的较小蛋白质能够自身作为puc转录的激活剂发挥作用,并且独立于其所在的大开放阅读框进行表达。

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