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首页> 外文期刊>Folia microbiologica >Optimization of a two-plasmid system for the identification of promoters recognized by RNA polymerase containing Mycobacterium tuberculosis stress response sigma factor, sigma(F)
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Optimization of a two-plasmid system for the identification of promoters recognized by RNA polymerase containing Mycobacterium tuberculosis stress response sigma factor, sigma(F)

机译:优化用于鉴定由含结核分枝杆菌应激反应sigma因子sigma(F)的RNA聚合酶识别的启动子的双质粒系统

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The previously established two-plasmid system in Escherichia coli for the identification of Mycobacterium tuberculosis promoters that are recognized by RNA polymerase containing the stress response sigma factor sigma(F) was optimized. Expression of the M. tuberculosis sigma(F) encoded by sigF gene was under the control of the isopropyl beta-D-thiogalactopyranoside (IPTG)-dependent P-trc promoter. A low level of IPTG induced a nontoxic but sufficient level of sigma(F) to interact with the core enzyme of RNA polymerase. Such an RNA polymerase holoenzyme recognized the known sigma(F)-dependent promoter, usfXp1, which was cloned in the compatible promoter probe plasmid, upstream of a promoterless lacZ alpha reporter gene. Primer extension analysis of the usfXp1 promoter in the E. coli two-plasmid system after IPTG-induced expression of M. tuberculosis sigF revealed a transcription start point that was identical as in M. tuberculosis. This new system has been shown to be useful for identification of M. tuberculosis sigma(F)-dependent promoters.
机译:优化了先前在大肠杆菌中建立的用于鉴定结核分枝杆菌启动子的两质粒系统,该结核分枝杆菌启动子被包含应力响应sigma因子sigma(F)的RNA聚合酶识别。 sigF基因编码的结核分枝杆菌sigma(F)的表达受异丙基β-D-硫代吡喃半乳糖吡喃糖苷(IPTG)依赖性P-trc启动子的控制。低水平的IPTG诱导了无毒但足够水平的sigma(F)与RNA聚合酶的核心酶相互作用。这种RNA聚合酶全酶识别已知的sigma(F)依赖性启动子usfXp1,该启动子克隆在兼容的启动子探针质粒中,无启动子lacZ alpha报告基因的上游。 IPTG诱导的结核分枝杆菌sigF表达后,usfXp1启动子在大肠杆菌两质粒系统中的引物延伸分析揭示了与结核分枝杆菌相同的转录起点。该新系统已显示可用于鉴定结核分枝杆菌sigma(F)依赖性启动子。

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