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Highly Efficient Modification of Bacterial Artificial Chromosomes (BACs) Using Novel Shuttle Vectors Containing the R6Kγ Origin of Replication

机译:高效人工修饰细菌人工染色体(BAC)使用新型穿梭载体包含R6Kγ复制的起源。

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摘要

Bacterial artificial chromosome (BAC) mediated transgenesis has proven to be a highly reliable way to obtain accurate transgene expression for in vivo studies of gene expression and function. A rate-limiting step in use of this technology to characterize large numbers of genes has been the process with which BACs can be modified by homologous recombination in Escherichia coli. We report here a highly efficient method for modifying BACs by using a novel set of shuttle vectors that contain the R6Kγ origin for DNA replication, the E. coli RecA gene for recombination, and the SacB gene for negative selection. These new vectors greatly increased the ease with which one can clone the shuttle vectors, as well as screen for co-integrated and resolved clones. Furthermore, we simplify the shuttle vector cloning to one step by incorporation of a “built-in” resolution cassette for rapid removal of the unwanted vector sequences. This new system has been used to modify a dozen BACs. It is well suited for efficient production of modified BACs for use in a variety of in vivo studies.
机译:细菌人工染色体(BAC)介导的转基因已被证明是获得准确的转基因表达以进行体内基因表达和功能研究的高度可靠的方法。使用该技术表征大量基因的限速步骤一直是通过在大肠杆菌中进行同源重组来修饰BAC的过程。我们在这里报告了一种高效的方法,通过使用一组新型的穿梭载体修饰BAC,其中的穿梭载体包含R6Kγ起点用于DNA复制,E。coli RecA基因用于重组以及SacB基因用于阴性选择。这些新载体大大增加了克隆穿梭载体的难度,并筛选了共同整合和分离的克隆。此外,我们通过引入“内置”解析盒将快速去除不需要的载体序列,将穿梭载体克隆简化为一个步骤。此新系统已用于修改许多BAC。它非常适合有效生产用于各种体内研究的修饰BAC。

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