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转录激活因子PrfA对单核细胞增生李斯特菌毒力基因的差异调控

Differential regulation of the virulence genes of Listeria monocytogenes by the transcriptional activator PrfA.

作者信息

Bohne J, Kestler H, Uebele C, Sokolovic Z, Goebel W

机构信息

Theodor-Boveri-Institut für Biowissenschaften der Universität Würzburg (Lehrstuhl für Mikrobiologie), Germany.

出版信息

Mol Microbiol. 1996 Jun;20(6):1189-98. doi: 10.1111/j.1365-2958.1996.tb02639.x.

Abstract

The two Listeria monocytogenes strains EGD and NCTC 7973 display a different regulation pattern of their PrfA-dependent genes. All PrfA-dependent genes from L. monocytogenes NCTC 7973 are much more efficiently transcribed in brain-heart infusion medium than those from strain EGD. Transcription of these genes in EGD is, however, induced after shift into Minimal Essential Medium (MEM) to a level that is comparable to that of strain NCTC 7973. Expression of the internalin gene (inlA) is also influenced by PrfA, but only one (P2) out of three mapped promoters is strictly dependent on PrfA. In contrast to the other PrfA-regulated genes, transcription of inlA even from the P2 promoter is reduced in both strains after shift to MEM. The prfA deletion mutant SLCC 53 complemented with multiple copies of prfA synthesizes large amounts of monocistronic prfA transcript, but there is no concomitant increase in the transcripts of the PrfA-dependent genes. However, upon a shift into MEM, transcription of the PrfA-dependent genes (with the exception of the inlA gene) is highly induced even in the absence of de novo protein synthesis. The PrfA proteins of the two studied L. monocytogenes strains differ in their ability to activate PrfA-dependent genes. This difference is probably the result of amino acid exchange(s) in the C-terminal part of these proteins. Strain EGD supplemented with multiple copies of prfA-7973 shows a similar regulation of the PrfA-dependent genes as strain NCTC 7973, whereas multiple copies of prfA-EGD introduced into strain EGD hardly change the rate of transcription of the PrfA-dependent genes. Our data thus suggest that PrfA-mediated gene expression depends not only on the amount of the PrfA protein and the 'quality' of the putative PrfA-binding sites, but also on the 'quality' of the PrfA protein which seems to be influenced by its amino acid composition and by environmental parameters.

摘要

两株单核细胞增生李斯特菌菌株EGD和NCTC 7973对其PrfA依赖性基因表现出不同的调控模式。来自单核细胞增生李斯特菌NCTC 7973的所有PrfA依赖性基因在脑心浸液培养基中的转录效率比来自EGD菌株的基因高得多。然而,EGD中这些基因的转录在转入最低限度基本培养基(MEM)后被诱导至与NCTC 7973菌株相当的水平。内化素基因(inlA)的表达也受PrfA影响,但三个定位启动子中只有一个(P2)严格依赖PrfA。与其他PrfA调控基因相反,转入MEM后,两株菌中即使是来自P2启动子的inlA转录也会减少。用多个prfA拷贝互补的prfA缺失突变体SLCC 53合成大量单顺反子prfA转录本,但PrfA依赖性基因的转录本没有相应增加。然而,转入MEM后,即使在没有从头蛋白质合成的情况下,PrfA依赖性基因(inlA基因除外)的转录也会被高度诱导。所研究的两株单核细胞增生李斯特菌菌株的PrfA蛋白在激活PrfA依赖性基因的能力上有所不同。这种差异可能是这些蛋白C末端部分氨基酸交换的结果。补充多个prfA - 7973拷贝的EGD菌株对PrfA依赖性基因的调控与NCTC 7973菌株相似,而导入EGD菌株的多个prfA - EGD拷贝几乎不改变PrfA依赖性基因的转录速率。因此,我们的数据表明,PrfA介导的基因表达不仅取决于PrfA蛋白的量和假定的PrfA结合位点的“质量”,还取决于PrfA蛋白的“质量”,而PrfA蛋白的“质量”似乎受其氨基酸组成和环境参数的影响。

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