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Creation of Golden Gate constructs for gene doctoring

机译:基因译者的Golden Gate构造的创建

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Gene doctoring is an efficient recombination-based genetic engineering approach to mutagenesis of the bacterial chromosome that combines the λ-Red recombination system with a suicide donor plasmid that is cleaved in vivo to generate linear DNA fragments suitable for recombination. The use of a suicide donor plasmid makes Gene Doctoring more efficient than other recombineering technologies. However, generation of donor plasmids typically requires multiple cloning and screening steps. We constructed a simplified acceptor plasmid, called pDOC-GG, for the assembly of multiple DNA fragments precisely and simultaneously to form a donor plasmid using Golden Gate assembly. Successful constructs can easily be identified through blue-white screening. We demonstrated proof of principle by inserting a gene for green fluorescent protein into the chromosome of Escherichia coli. We also provided related genetic parts to assist in the construction of mutagenesis cassettes with a tetracycline-selectable marker. Our plasmid greatly simplifies the construction of Gene Doctoring donor plasmids and allows for the assembly of complex, multi-part insertion or deletion cassettes with a free choice of target sites and selection markers. The tools we developed are applicable to gene editing for a wide variety of purposes in Enterobacteriaceae and potentially in other diverse bacterial families.
机译:基因博士是一种高效的重组基因工程方法,可诱变细菌染色体,其将λ-红色重组系统与自杀式供体质粒相结合,其在体内切割以产生适合重组的线性DNA片段。使用自杀式供体质粒使基因篡改比其他重组技术更有效。然而,供体质粒的产生通常需要多种克隆和筛选步骤。我们构建了一种称为PDOC-GG的简化受体质粒,用于精确地且同时形成具有金色栅极组件的供体质粒的组装。通过蓝白筛选可以轻松识别成功的构造。我们通过将绿色荧光蛋白基因插入大肠杆菌染色体来证明原理的证据。我们还提供了相关的遗传零件,以帮助用四环素可选择的标记构建诱变盒。我们的质粒极大地简化了基因篡改供体质粒的构建,并允许组装复杂的多部分插入或删除盒,并选择靶位点和选择标记。我们开发的工具适用于基因编辑在肠杆菌薄膜中的各种目的,并且可能在其他不同的细菌家庭中。

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