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志贺氏菌毒力的温度调节:阻遏基因virR的鉴定,hns的类似物,以及酪氨酸转移RNA(tRNA1(Tyr))的部分互补作用。

Temperature regulation of Shigella virulence: identification of the repressor gene virR, an analogue of hns, and partial complementation by tyrosyl transfer RNA (tRNA1(Tyr)).

作者信息

Hromockyj A E, Tucker S C, Maurelli A T

机构信息

Department of Microbiology, Uniformed Services University of the Health Sciences, Bethesda, Maryland 20814-4799.

出版信息

Mol Microbiol. 1992 Aug;6(15):2113-24. doi: 10.1111/j.1365-2958.1992.tb01385.x.

Abstract

virR is the central regulatory locus required for coordinate temperature-regulated virulence gene expression in the human enteric pathogens of Shigella species. Detailed characterization of VirR+ clones revealed that virR consisted of a 411 bp open reading frame (ORF) that mapped to a chromosomally located 1.8kb EcoRI-AccI DNA fragment from Shigella flexneri. Insertional inactivation of the virR ORF at a unique HpaI restriction site resulted in a loss of VirR+ activity. The virR ORF nucleotide sequence was virtually identical to the Escherichia coli hns gene, which encodes the histone-like protein, H-NS. Based on the predicted amino acid sequence of E. coli H-NS, only a single conservative base-pair change was identified in the virR gene. An additional clone, designated VirRP, which only partially complemented the virR mutation, was also characterized and determined by Southern hybridization and nucleotide sequence analysis to be unique from virR. Subclone mapping of this clone indicated that the VirRP phenotype was a result of the multiple copy expression of the S. flexneri gene for tRNA(Tyr). These data constitute the first direct genetic evidence that virR is an analogue of the E. coli hns gene, and suggest a model for temperature regulation of Shigella species virulence via the bacterial translational machinery.

摘要

virR是志贺氏菌属人类肠道病原体中协调温度调节的毒力基因表达所需的核心调节位点。对VirR+克隆的详细表征表明,virR由一个411 bp的开放阅读框(ORF)组成,该阅读框定位于来自福氏志贺氏菌的染色体定位的1.8kb EcoRI-AccI DNA片段上。在独特的HpaI限制性位点对virR ORF进行插入失活导致VirR+活性丧失。virR ORF核苷酸序列与编码类组蛋白H-NS的大肠杆菌hns基因几乎相同。根据大肠杆菌H-NS的预测氨基酸序列,在virR基因中仅鉴定出一个保守的碱基对变化。另一个名为VirRP的克隆,仅部分互补virR突变,也通过Southern杂交和核苷酸序列分析进行了表征,并确定其与virR不同。该克隆的亚克隆定位表明,VirRP表型是福氏志贺氏菌tRNA(Tyr)基因多拷贝表达的结果。这些数据构成了virR是大肠杆菌hns基因类似物的确切直接遗传证据,并提出了一种通过细菌翻译机制对志贺氏菌属毒力进行温度调节的模型。

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