摘要
试验构建牛朊蛋白(prion protein,PRNP)基因的真核表达载体,为进一步研究牛朊蛋白的生理功能和从细胞水平研究抗疯牛病转基因克隆牛奠定基础。采用重叠延伸PCR(splicing overlap extension PCR,SOE-PCR)法扩增获得牛PRNP基因序列,并克隆到带有DsRED2报告基因的真核表达载体pDsRED2-N1中,将双酶切、PCR、测序鉴定的阳性质粒经脂质体转染牛骨髓间充质干细胞(BMSC);通过荧光显微镜观察转染细胞,并用800μg/mL G418对转染的细胞进行药物筛选。琼脂糖凝胶电泳显示基因合成的片段大小和构建的载体大小与预期相符;重组表达载体转染BMSC后有红色荧光出现;通过药物筛选出了稳定转染的细胞单克隆。通过SOE-PCR成功扩增了牛PRNP基因序列,并构建成真核表达载体,得到稳定表达目的蛋白的BMSC细胞。
In order to further study the physiological function of bovine prion protein and anti mad cow disease cloned transgenic cattle basis form cellular level, we constructed a bovine prion protein gene (PRNP) eukaryotic expression vector. The PRNP gene was cloned by splicing overlap extension PCR (SQE-PCR) method, and inserted into the report with DsRED2 eukaryotic vector pDsRED2-N1. This recombinant plasmid pDsRED2-N1 was identified by digestion of endonuclease, PCR and sequencing. Then, it was transfected into bovine BMSC cell line mediated by LipofeetarnineTa2000. The transfeeted cells was detected by fluorescence microscopy and drug screening by 800μg/mL G418. Electrophoresis analysis showed that the se- quences were amplified and the sizes of products were accord with expectation. The recombinant plasrnid was expressed in BMSC. The positive single stable transfection cell clones were also got by drug screening. The PRNP gene had been cloned by splicing overlap extension PCR method, and the recombinant eukaryotie vector stable expressed in BMSC successfully.
出处
《中国畜牧兽医》
CAS
北大核心
2012年第7期20-25,共6页
China Animal Husbandry & Veterinary Medicine
基金
国家"抗病转基因牛新品种培育"项目资助(2008ZX08007-004)
