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Improved Plasmid-Based System for Fully Regulated Off-To-On Gene Expression in Escherichia coli: Application to Production of Toxic Proteins

机译:改善基于质粒的系统用于大肠杆菌的完全核对基因表达:毒性蛋白的生产应用

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摘要

In previous work transduction of Escherichia coli with phage λ particles carrying packaged plasmids was shown to provide complete off-to-on expression of plasmid-borne genes (. J. Bacteriol. 185, 6522–6529). The plasmids used contained the phage λcos site (and hence are cosmids) and were very efficiently packaged into λ phage particles in vivo upon induction of λ lysogens having an inactivated cos site. However, a shortcoming was that the stocks contained a variable fraction of infectious λ phage which arose by recombinational repair of the inactive cos site. I report that the construction of E. coli strains that eliminate the background of infectious phage and show that the system can be utilized to express proteins by the phage T7 RNA polymerase/pET vector system.
机译:在以前的工作中,用携带包装好的质粒的噬菌体λ质粒转导大肠杆菌被证明可以完整地表达质粒携带的基因(。J. Bacteriol。185,6522–6529)。所使用的质粒包含噬菌体的λcos位点(因此是粘粒),并且在诱导具有灭活的cos位点的λ溶原菌后,在体内非常有效地包装到λ噬菌体颗粒中。但是,缺点是这些种群包含可变比例的传染性λ噬菌体,这些噬菌体是通过对无活性的cos位点进行重组修复而产生的。我报告说,大肠杆菌菌株的构建消除了感染性噬菌体的背景,并表明该系统可用于噬菌体T7 RNA聚合酶/ pET载体系统表达蛋白质。

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