应用反向PCR克隆慢病毒介导的转基因小鼠整合位点序列

目的：为分析慢病毒介导的转基因小鼠中外源基因整合位点的信息,应用反向PCR克隆整合位点序列。方法：小鼠基因组总DNA酶解和自连接后,针对慢病毒载体的特点在LTR附近设计一组特异的PCR引物,优化半巢式PCR的各种参数,提高整合位点序列克隆的效率。结果：克隆了分别携带绿色荧光蛋白（GFP）和转铁蛋白（TF）基因的慢病毒介导的转基因小鼠家系7只小鼠中10个外源基因整合位点序列。结论：本方法可用于慢病毒介导的转基因小鼠整合位点序列的克隆,为分析整合位点与外源基因表达之间的关系等提供了科学依据。

Molecular Cloning of the Sequences of Integration Sites in Transgenic Mice Mediated with Lentiviral Vectors Using Inverse PCR Approach

Objective： To investigate the information of transgene integrations in mice mediated with lentiviral vectors, the inverse PCR was used to clone the sequences of integration sites. Methods： The genomic DNA of the transgenic mice was digested with restriction endonuclease, followed by self-liagtion. A group of specific PCR primers were designed ac- cording to the characteristics of LTR and the flanking sequences of lentiviral vectors, and parameters of the semi-nested PCR were optimized. The cloning efficiency of sequences of the integration sites was improved. Results： Ten DNA se- quences of the integration sites in 7 lentivrial mice carrying GFP or TF （transferrin） gene were cloned successfully. Con- clusion： The method described in this article was suitable for cloning the sequences of integration sites, which will provide scientific data for the studies of the relationship between integration sites and transgene expression.