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A recombineering based approach for high-throughput conditional knockout targeting vector construction

机译:基于重组的高通量条件敲除靶向载体构建方法

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摘要

Functional analysis of mammalian genes in vivo is primarily achieved through analysing knockout mice. Now that the sequencing of several mammalian genomes has been completed, understanding functions of all the genes represents the next major challenge in the post-genome era. Generation of knockout mutant mice has currently been achieved by many research groups but only by making individual knockouts, one by one. New technological advances and the refinements of existing technologies are critical for genome-wide targeted mutagenesis in the mouse. We describe here new recombineering reagents and protocols that enable recombineering to be carried out in a 96-well format. Consequently, we are able to construct 96 conditional knockout targeting vectors simultaneously. Our new recombineering system makes it a reality to generate large numbers of precisely engineered DNA constructs for functional genomics studies.
机译:体内哺乳动物基因的功能分析主要是通过分析基因敲除小鼠来实现的。现在已经完成了几个哺乳动物基因组的测序,了解所有基因的功能代表了后基因组时代的下一个重大挑战。目前,许多研究小组已经实现了基因敲除突变小鼠的产生,但是只能通过逐个进行个体敲除来实现。新技术的进步和现有技术的完善对小鼠全基因组靶向诱变至关重要。我们在这里描述了使重组能够以96孔格式进行的新重组试剂和方案。因此,我们能够同时构建96个条件敲除靶向载体。我们新的重组系统使为功能基因组学研究生成大量经过精确工程改造的DNA构建体成为现实。

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