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作 者:于峰祥[1] 于建宁[2] 王公金[1,2] 潘伟芹[1] 徐小波[2] 徐志伟[3] 花卫华[3] 刘泉[3]
机构地区:[1]南京师范大学医学分子生物学重点实验室,江苏南京210097 [2]江苏省农业科学院畜牧研究所,江苏南京210014 [3]江苏丘陵地区镇江农业科学研究所,江苏句容212400
出 处:《江苏农业学报》2011年第5期1043-1046,共4页Jiangsu Journal of Agricultural Sciences
基 金:农业部转基因生物新品种培育重大专项(2008ZX08006-004);江苏省农业科技自主创新基金项目[CX(10)421]
摘 要:探讨SQR基因真核表达载体pcDNA3.1(-)-SQR-Myc的构建及其在真核细胞中的表达。根据已知荚膜红杆菌SQR基因序列设计5'端和3'端引物,采用PCR方法获得SQR基因,通过pMD-18T载体构建得到中间质粒pMD-18T-SQR-Myc;采用限制性内切酶XhoⅠ和KpnⅠ双酶切该中间质粒,将SQR基因插入真核表达载体pcD-NA3.1(-)相应酶切位点,获得重组质粒pcDNA3.1(-)-SQR-Myc;采用脂质体法瞬时转染HEK293细胞并进行West-ern blot蛋白鉴定。结果显示:该研究已成功构建了真核表达载体pcDNA3.1(-)-SQR-Myc,质粒测序及酶切结果完全正确,并且SQR能够在HEK293细胞系中正常表达。To construct the eukaryotic vector pcDNA3.1(-)-SQR-Myc and investigate its expression in eukaryocyte,the 5′ primers and 3′ primers were designed and synthesized following the gene sequence of SQR from Rhodobacter capsulatus.The sulfide-quinone reductase(SQR)gene was obtained by PCR and the intermediate vector pMD-18T-SQR-Myc was constructed.The vector was then digested by restriction enzymes XhoⅠand KpnⅠ,and the SQR gene was inserted into the the corresponding restriction enzyme cutting site to construct recombinant plasmid pcDNA3.1(-)-SQR-Myc.The plasmid pcDNA3.1(-)-SQR-Myc was transiently transfected into the HEK293 cells with lipidosome and identified by Western blotting.The results showed that the eukaryotic vector pcDNA3.1(-)-SQR-Myc was constructed successfully,which was confirmed by restriction enzyme digestion and sequencing.Western blotting revealed that SQR could be expressed in HEK293 cells.
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