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作 者:杨发建[1] 张琴[1] 何芸[1] 周龙洋[1] 卜友泉[2] 孙文娟[1] 何百成[1] 杨俊霞[1]
机构地区:[1]重庆医科大学药理学教研室,重庆400016 [2]重庆医科大学生物化学与分子生物学教研室,重庆400016
出 处:《中国生物制品学杂志》2013年第4期465-468,共4页Chinese Journal of Biologicals
基 金:国家自然科学基金资助项目(30600812)
摘 要:目的构建胰岛素诱导基因-2(Insulin induced gene-2,Insig-2)启动子荧光素酶报告基因重组质粒,并检测其转录活性。方法从人基因组DNA中扩增Insig-2基因转录起始位点上游1 389 bp的启动子片段,插入pGL3-basic质粒中,构建重组质粒pGL3-Insig-2,将其与内参质粒pRL-TK瞬时共转染HEK293、HepG2和3T3-L1细胞,采用双荧光素酶法检测Insig-2启动子活性。结果重组质粒pGL3-Insig-2经双酶切和DNA测序,证实构建正确;pGL3-Insig-2质粒在HEK293、HepG2和3T3-L1细胞中均具有启动子活性,分别为阴性对照组(pGL3-basic空载体)的28、40和214倍、阳性对照组(pGL3-SV40)的2.6、5.5和30倍,呈现出强启动子活性。结论成功构建了Insig-2基因启动子荧光素酶报告基因重组质粒,为后续Insig-2基因的深入研究奠定了基础。Objective To construct the recombinant plasmid containing human insulin induced gene-2(Insig-2) promoter luciferase reporter,and determine its transcriptional activity.Methods The promoter fragment at a length of 1 389 bp upstream at transcription site of insig-2 gene was amplified by PCR from human genomic DNA and inserted into vector pGL3-basic.The constructed recombinant plasmid pGL3-Insig-2 and internal reference plasmid pRL-TK were transiently co-transfected to HEK293,HepG2 and 3T3-L1 cells,and determined for Insig-2 promoter activity by dual-luciferase reporter assay.Results Restriction analysis and sequencing proved that recombinant plasmid pGL3-Insig-2 was constructed correctly.The recombinant plasmid showed promoter activity in HEK293,HepG2 and 3T3-L1 cells,which were 28,40 and 214 times of those in negative control group(empty vector pGL3-basic) and 2.6,5.5 and 30 times of those in positive control group(pGL3-SV40),respectively.Conclusion Recombinant plasmid containing Insig-2 promoter luciferase reporter was successfully constructed,which laid a foundation of further study on the gene.
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