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Establishment of an efficient BAC transgenesis protocol and its application to functional characterization of the mouse Brachyury locus

机译:有效的BAC转基因协议的建立及其在小鼠Brachyury基因座功能表征中的应用

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Transgenesis using large DNA such as YAC or BAC has extended the range of applications in functional genomics. Here we describe an efficient BAC transgenesis protocol using a simple BAC DNA preparation method adopted from YAC DNA purification methods. This method allowed us to isolate BAC DNA from small scale culture of BAC-containing cells in sufficient quantity and purity for microinjection. More than 40 founders have been produced with linearized BAC DNA prepared by this method, and 85% of them contained intact BAC transgenes. In contrast, when circular BAC DNA was injected, an approximately three-fold reduction of transgene integration rate was observed and fewer intact transgene integrations were obtained. A line of transgenic mice carrying a 170-kb BAC clone generated in this way successfully rescued tail and embryonic lethality phenotypes of the mouse Brachyury (T) mutants, further demonstrating the utility of this method in functional analysis of the mouse genome.
机译:使用大型DNA(例如YAC或BAC)进行转基因已扩展了功能基因组学的应用范围。在这里,我们描述了一种有效的BAC转基因方案,它使用了从YAC DNA纯化方法中采用的简单BAC DNA制备方法。这种方法使我们能够从微量培养的含BAC细胞的小规模培养物中分离出BAC DNA,其数量和纯度足以进行显微注射。用这种方法制备的线性化BAC DNA已经产生了40多个创始人,其中有85%的人包含完整的BAC转基因。相反,当注射环状BAC DNA时,观察到转基因整合率降低了大约三倍,并且获得的完整转基因整合较少。携带以这种方式生成的170 kb BAC克隆的转基因小鼠系成功拯救了小鼠Brachyury(T)突变体的尾巴和胚胎致死表型,进一步证明了该方法在小鼠基因组功能分析中的实用性。

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