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An improved Red/ET recombineering system and mouse ES cells culture conditions for the generation of targeted mutant mice

机译:一种改进的红色/等重组系统和小鼠ES细胞培养条件用于产生靶向突变小鼠

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Targeted mutant mice generated on a C57BL/6 background are powerful tools for analysis of the biological functions of genes, and gene targeting technologies using mouse embryonic stem (ES) cells have been used to generate such mice. Recently, a bacterial artificial chromosome (BAC) recombineering system was established for the construction of targeting vectors. However, gene retrieval from BACs for the generation of gene targeting vectors using this system remains difficult. Even when construction of a gene targeting vector is successful, the efficiency of production of targeted mutant mice from ES cells derived from C57BL/6 mice are poor. Therefore, in this study, we first improved the strategy for the retrieval of genes from BACs and their transfer into a DT-A plasmid, for the generation of gene targeting vectors using the BAC recombineering system. Then, we attempted to generate targeted mutant mice from ES cell lines derived from C57BL/6 mice, by culturing in serum-free medium. In conclusion, we established an improved strategy for the efficient generation of targeted mutant mice on a C57BL/6 background, which are useful for the in vivo analysis of gene functions and regulation.
机译:在C57BL / 6背景上产生的靶向突变小鼠是用于分析基因生物学功能的强大工具,并且使用使用小鼠胚胎茎(ES)细胞的基因靶向技术已经用于产生这种小鼠。最近,建立了一种用于构建靶向载体的细菌人工染色体(BAC)重组系统。然而,使用该系统的基因从BAC获取基因靶向载体的基因仍然困难。即使当靶向载体的基因的构建成功时,衍生自C57BL / 6小鼠的ES细胞的靶向突变小鼠的生产效率也是差。因此,在本研究中,我们首先改善了从BAC的基因检索的策略及其转移到DT-A质粒中,用于使用BAC重组系统产生基因靶向载体。然后,通过在无血清培养基中培养,我们试图从衍生自C57BL / 6小鼠的ES细胞系产生靶向突变小鼠。总之,我们在C57BL / 6背景下建立了有效生成靶向突变小鼠的改善策略,这对于基因功能和调节的体内分析有用。

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