首页> 外文期刊>Journal of applied microbiology >Development of the recombinase-based in vivo expression technology in Streptococcus thermophilus and validation using the lactose operon promoter.
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Development of the recombinase-based in vivo expression technology in Streptococcus thermophilus and validation using the lactose operon promoter.

机译:嗜热链球菌中基于重组酶的体内表达技术的开发以及使用乳糖操纵子启动子的验证。

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Aims: To construct and validate the recombinase-based in vivo expression technology (R-IVET) tool in Streptococcus thermophilus (ST). Methods and Results: The R-IVET system we constructed in the LMD-9 strain includes the plasmid pULNcreB allowing transcriptional fusion with the gene of the site-specific recombinase Cre and the chromosomal cassette containing a spectinomycin resistance gene flanked by two loxP sites. When tested in M17 medium, promoters of the genes encoding the protease PrtS, the heat-shock protein Hsp16 and of the lactose operon triggered deletion of the cassette, indicating promoter activity in these conditions. The lactose operon promoter was also found to be activated during the transit in the murine gastrointestinal tract. Conclusions: The R-IVET system developed in ST is relatively stable, functional, very sensitive and can be used to assay activity of promoters, which are specifically active in in vivo conditions. Significance and Impact of the Study: This first adaptation of R-IVET to ST provides a highly valuable tool allowing an exploration of the physiological state of ST in the GIT of mammals, fermentation processes or dairy products.
机译:目的:构建和验证嗜热链球菌(ST)中基于重组酶的体内表达技术(R-IVET)工具。方法和结果:我们在LMD-9菌株中构建的R-IVET系统包括质粒pULNcreB,该质粒可与位点特异性重组酶Cre的基因转录融合,而染色体盒则包含侧翼有两个loxP位点的壮观霉素抗性基因。在M17培养基中测试时,编码蛋白酶PrtS,热休克蛋白Hsp16和乳糖操纵子的基因的启动子触发了盒的缺失,表明启动子在这些条件下具有活性。还发现乳糖操纵子启动子在鼠胃肠道中转运期间被激活。结论:ST开发的R-IVET系统相对稳定,功能正常,非常灵敏,可用于检测启动子的活性,这些启动子在体内条件下具有特异性。研究的意义和影响:R-IVET对ST的首次适应提供了一种非常有价值的工具,可用于探索哺乳动物GIT,发酵过程或乳制品中ST的生理状态。

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