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鼠伤寒沙门氏菌毒力质粒编码一种质粒编码毒力基因的正调控因子。

The Salmonella typhimurium virulence plasmid encodes a positive regulator of a plasmid-encoded virulence gene.

作者信息

Caldwell A L, Gulig P A

机构信息

Department of Immunology and Medical Microbiology, University of Florida College of Medicine, Gainesville 32610-0266.

出版信息

J Bacteriol. 1991 Nov;173(22):7176-85. doi: 10.1128/jb.173.22.7176-7185.1991.

Abstract

The 90-kb virulence plasmid of Salmonella typhimurium is necessary for invasion beyond the Peyer's patches to the mesenteric lymph nodes and spleens of orally inoculated mice. Two Tn5 insertions located on the left side of a previously identified 14-kb virulence region (P. A. Gulig and R. Curtiss III, Infect. Immun. 58:3262-3271, 1988) and mapping 272 bp from each other exhibited opposite effects on splenic infection of mice after oral inoculation. spvR23::Tn5 decreased splenic infection by 1,000-fold, whereas a spv-14::Tn5 mutant outcompeted wild-type S. typhimurium for splenic infection by 27-fold in mice fed mixtures of mutated and wild-type S. typhimurium. spvR23::Tn5 was complemented by a virulence plasmid subclone with an insert sequence encoding only an 891-bp open reading frame specifying a 33,000-molecular-weight protein. The amino acid sequence of this open reading frame had significant homology to members of the LysR family of positive regulatory proteins; thus, the gene was named spvR (salmonella plasmid virulence). To examine the possible regulatory effects of spvR on other virulence genes, we constructed a lacZ operon fusion in a downstream virulence gene, spvB. When spvR subcloned behind the lac promoter was provided on a separate plasmid in trans to the spvB-lacZ operon fusion, transcription of spvB increased 15-fold. spv-14::Tn5, which conferred a competitive advantage to S. typhimurium, increased the expression of a spvR-lacZ operon fusion in cis. spvR is therefore a positive regulator of spvB and an essential virulence gene of S. typhimurium. As opposed to having spvR subcloned behind the lac promoter, the wild-type spvR gene present on the virulence plasmid did not function to positively regulate spvB-lacZ in trans when salmonellae were grown to the log phase in L broth, suggesting that this regulatory system is activated in vivo during infection.

摘要

鼠伤寒沙门氏菌90kb的毒力质粒对于经口接种的小鼠从派伊尔氏结侵袭至肠系膜淋巴结和脾脏是必需的。位于先前鉴定的14kb毒力区域左侧(P.A.古利格和R.柯蒂斯三世,《感染与免疫》58:3262 - 3271,1988)且彼此间相距272bp的两个Tn5插入片段,在经口接种后对小鼠脾脏感染呈现出相反的影响。spvR23::Tn5使脾脏感染降低了1000倍,而在给小鼠投喂突变型和野生型鼠伤寒沙门氏菌混合物时,spv - 14::Tn5突变体在脾脏感染方面比野生型鼠伤寒沙门氏菌更具竞争力,其感染能力是野生型的27倍。spvR23::Tn5可被一个毒力质粒亚克隆所互补,该亚克隆的插入序列仅编码一个891bp的开放阅读框,该开放阅读框编码一种分子量为33000的蛋白质。此开放阅读框的氨基酸序列与正调控蛋白的LysR家族成员具有显著同源性;因此,该基因被命名为spvR(沙门氏菌质粒毒力)。为了研究spvR对其他毒力基因可能的调控作用我们在下游毒力基因spvB中构建了一个lacZ操纵子融合体。当在与spvB - lacZ操纵子融合体反式存在的单独质粒上提供位于lac启动子下游亚克隆的spvR时,spvB的转录增加了15倍。赋予鼠伤寒沙门氏菌竞争优势的spv - 14::Tn5顺式增加了spvR - lacZ操纵子融合体的表达。因此,spvR是spvB的正调控因子,也是鼠伤寒沙门氏菌的一个必需毒力基因。与将spvR亚克隆于lac启动子下游不同,当沙门氏菌在L肉汤中生长至对数期时,毒力质粒上存在的野生型spvR基因在反式情况下不能对spvB - lacZ起到正调控作用,这表明该调控系统在感染过程中于体内被激活。

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