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单核细胞增生李斯特菌中prfA依赖性调控的inlC启动子上的一些必需元件。

Some essential elements on the inlC promoter for prfA-dependent regulation in Listeria monocytogenes.

作者信息

Luo Qin, Zhou Qing-Chun, Deng Ling-fu, Gao Qiang, Liu De-li

机构信息

College of Life Science, Central China Normal University, Wuhan 430079, China.

出版信息

Wei Sheng Wu Xue Bao. 2007 Feb;47(1):22-8.

PMID:17436618
Abstract

To study some essential elements of a PrfA-dependent promoter of Listeria monocytogenes, a series of promoter mutants incorporated into upstream of a promoterless lacZ gene were constructed from a known listerial PrfA-dependent promoter, inlC promoter, by PCR-mediated site-directed mutagenesis and recombinant PCR technique and then electroporated into L. monocytogenes wild-type strain P14, prfA * mutant Pl4a and prfA deletion mutant A42. The corresponding transcription activities of altered promoters were measured by the beta-galactosidase assay. The results showed that a PrfA-box-like sequence ("pseudo-PrfA-box"), TTAACAGCGTTTGTTAA, 22bp downstream of the transcriptional start site of PinlC had no ability to enhance or inhibit the PrfA-dependent transcription of inlC promoter, even it was modified to the "ideal PrfA-box" TTAACATTTGTTAA. However, there was almost no PrfA-dependent transcriptional activity from the mutants deletion of the inlC original PrfA-box. Moreover, altered spacing between 3'-end of the PrfA-box and 5'-end of the -10 box in the inlC promoter region affected transcription efficiency dramatically, which also happened in another promoter-dependent promoter, plcA promoter. Those above suggested that besides the "PrfA-box", additional unknown PrfA-dependent promoter structure(s) or sequence(s) might be required for the PrfA binding to the promoter and initiation of transcription. Furthermore, the distance between the PrfA-box and the -10 box should be fixed to 22 or 23bp for the PrfA-dependent transcription.

摘要

为了研究单核细胞增生李斯特菌中依赖PrfA的启动子的一些关键元件,通过PCR介导的定点诱变和重组PCR技术,从已知的李斯特菌依赖PrfA的启动子inlC启动子构建了一系列整合到无启动子lacZ基因上游的启动子突变体,然后电穿孔导入单核细胞增生李斯特菌野生型菌株P14、prfA *突变体Pl4a和prfA缺失突变体A42。通过β-半乳糖苷酶测定法测量改变后的启动子的相应转录活性。结果表明,PinlC转录起始位点下游22bp处的一个类似PrfA框的序列(“假PrfA框”)TTAACAGCGTTTGTTAA没有增强或抑制inlC启动子依赖PrfA转录的能力,即使它被修饰为“理想PrfA框”TTAACATTTGTTAA。然而,缺失inlC原始PrfA框的突变体几乎没有依赖PrfA的转录活性。此外,inlC启动子区域中PrfA框的3'端与-10框的5'端之间的间隔改变显著影响转录效率,这在另一个依赖启动子的启动子plcA启动子中也发生。上述结果表明,除了“PrfA框”之外,PrfA与启动子结合及转录起始可能还需要其他未知的依赖PrfA的启动子结构或序列。此外,PrfA框与-10框之间的距离应为22或23bp才能实现依赖PrfA的转录。

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