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Improved Strains and Plasmid Vectors for Conditional Overexpression of His-Tagged Proteins in Haloferax volcanii

机译:改进的菌株和质粒载体,用于火山卤青中his标记蛋白的条件性过表达

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摘要

Research into archaea will not achieve its full potential until systems are in place to carry out genetics and biochemistry in the same species. Haloferax volcanii is widely regarded as the best-equipped organism for archaeal genetics, but the development of tools for the expression and purification of H. volcanii proteins has been neglected. We have developed a series of plasmid vectors and host strains for conditional overexpression of halophilic proteins in H. volcanii. The plasmids feature the tryptophan-inducible p.tnaA promoter and a 6xHis tag for protein purification by metal affinity chromatography. Purification is facilitated by host strains, where pitA is replaced by the ortholog from Natronomonas pharaonis. The latter lacks the histidine-rich linker region found in H. volcanii PitA and does not copurify with His-tagged recombinant proteins. We also deleted the mrr restriction endonuclease gene, thereby allowing direct transformation without the need to passage DNA through an Escherichia coli dam mutant.
机译:在建立对同一物种进行遗传学和生物化学的系统之前,对古细菌的研究将无法充分发挥其潜力。Haloferax volcanii被广泛认为是古细菌遗传学中装备最好的生物,但用于表达和纯化H. volcanii蛋白的工具的开发却被忽视了。我们开发了一系列质粒载体和宿主菌株,用于火山嗜盐蛋白的条件性过表达。该质粒具有色氨酸诱导的p.tnaA启动子和6xHis标签,用于通过金属亲和层析纯化蛋白质。宿主菌株促进纯化,其中 pitA 被来自 Natronomonas pharaonis 的直系同源物取代。后者缺乏在火山杆菌 PitA 中发现的富含组氨酸的连接子区域,并且不与 His 标记的重组蛋白共纯化。我们还删除了 mrr 限制性核酸内切酶基因,从而允许直接转化,而无需通过大肠杆菌坝突变体传代 DNA。

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