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葡萄球菌质粒pGO1上接合转移基因的TrsN转录调控

Transcriptional regulation by TrsN of conjugative transfer genes on staphylococcal plasmid pGO1.

作者信息

Sharma V K, Johnston J L, Morton T M, Archer G L

机构信息

Department of Medicine, Medical College of Virginia, Virginia Commonwealth University, Richmond 23298-0049.

出版信息

J Bacteriol. 1994 Jun;176(12):3445-54. doi: 10.1128/jb.176.12.3445-3454.1994.

DOI:10.1128/jb.176.12.3445-3454.1994
PMID:8206820
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC205530/
Abstract

The major conjugative transfer gene cluster of staphylococcal plasmid pGO1 (trs) consists of 13 open reading frames (trsA to trsM) transcribed from one DNA strand and a single 189-bp open reading frame (trsN) within the first 348 bp of trs that is transcribed divergently. Promoter regions for trsN and trsA partially overlap. TrsN, a 7,181-Da protein, was purified as a fusion to glutathione S-transferase and found to have DNA-binding activity. Increasing concentrations of the fusion protein progressively retarded the gel migration of PCR-generated DNA fragments containing predicted promoters 5' to trsL, trsA, and trsN. The target sequences contained areas of identity, including regions of dyad symmetry, that were protected in DNase I footprinting studies. The binding of TrsN to its trsL target was required for this target DNA to be stably introduced into Staphylococcus aureus on a high-copy-number vector. Provision of excess TrsN from this high-copy-number vector in S. aureus decreased beta-galactosidase activity from a trsL-lacZ transcriptional fusion and decreased pGO1 conjugation frequency. Conversely, both transcription and conjugation increased in the presence of excess trsL target. We propose that TrsN negatively regulates the transcription of genes essential for conjugative transfer by binding to regions 5' to their translational start sites.

摘要

葡萄球菌质粒pGO1的主要接合转移基因簇(trs)由13个从一条DNA链转录的开放阅读框(trsA至trsM)以及trs前348 bp内一个189 bp的单一开放阅读框(trsN)组成,trsN转录方向相反。trsN和trsA的启动子区域部分重叠。TrsN是一种7181 Da的蛋白质,作为与谷胱甘肽S-转移酶的融合蛋白被纯化,并发现具有DNA结合活性。融合蛋白浓度的增加逐渐阻碍了含有trsL、trsA和trsN预测启动子5'端的PCR扩增DNA片段在凝胶中的迁移。靶序列包含相同区域,包括在DNA酶I足迹研究中受到保护的二元对称区域。TrsN与其trsL靶标的结合是该靶标DNA在高拷贝数载体上稳定导入金黄色葡萄球菌所必需的。在金黄色葡萄球菌中,从该高拷贝数载体提供过量的TrsN会降低trsL-lacZ转录融合的β-半乳糖苷酶活性,并降低pGO1的接合频率。相反,在存在过量trsL靶标的情况下,转录和接合均增加。我们提出,TrsN通过结合到翻译起始位点5'端区域来负调控接合转移所需基因的转录。

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