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Application of Escherichia coli phage K1E DNA-dependent RNA polymerase for in vitro RNA synthesis and in vivo protein production in Bacillus megaterium

机译:大肠杆菌噬菌体K1E DNA依赖性RNA聚合酶在巨大芽孢杆菌体外RNA合成和体内蛋白质生产中的应用

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摘要

Gene "7" of Escherichia coli phage K1E was proposed to encode a novel DNA-dependent RNA polymerase (RNAP). The corresponding protein was produced recombinantly, purified to apparent homogeneity via affinity chromatography, and successfully employed for in vitro RNA synthesis. Optimal assay conditions (pH 8, 37°C, 10 mM magnesium chloride and 1.3 mM spermidine) were established. The corresponding promoter regions were identified on the phage genome and summarized in a sequence logo. Surprisingly, next to K1E promoters, the SP6 promoter was also recognized efficiently in vitro by K1E RNAP, while the T7 RNAP promoter was not recognized at all. Based on these results, a system for high-yield in vitro RNA synthesis using K1E RNAP was established. The template plasmid is a pUC18 derivative, which enables blue/white screening for positive cloning of the target DNA. Production of more than 5 μg of purified RNA per microgram plasmid DNA was achieved. Finally, in vivo protein production systems for Bacillus megaterium were established based on K1E and SP6 phage RNAP transcription. Up to 61.4 mg g _(CDW)~(-1) (K1E RNAP) of the reporter protein Gfp was produced in shaking flask cultures of B. megaterium.
机译:提出了大肠杆菌噬菌体K1E的基因“ 7”编码一种新型的DNA依赖性RNA聚合酶(RNAP)。重组产生相应的蛋白质,通过亲和色谱纯化至表观同质,并成功用于体外RNA合成。确定了最佳测定条件(pH 8、37°C​​,10 mM氯化镁和1.3 mM亚精胺)。在噬菌体基因组上鉴定出相应的启动子区域,并概括在序列标志中。令人惊讶的是,在K1E启动子旁边,SP6启动子也被K1E RNAP高效地识别出来,而T7 RNAP启动子根本没有被识别。基于这些结果,建立了使用K1E RNAP进行高产率体外RNA合成的系统。模板质粒是pUC18衍生物,可进行蓝/白筛选以阳性克隆目标DNA。每个微克质粒DNA产生超过5μg的纯化RNA。最后,基于K1E和SP6噬菌体RNAP转录,建立了巨大芽孢杆菌的体内蛋白质生产系统。在巨大芽孢杆菌的摇瓶培养物中产生了高达61.4 mg g_(CDW)〜(-1)(K1E RNAP)的报道蛋白Gfp。

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