转座子piggyBac介导的HSV-tk基因在妇科恶性肿瘤细胞中长期稳定表达的研究  被引量：3

作　　者：康玉[1] 孙庆文[2] 余文博[2] 程明军[1] 张晓燕[1] 武欣[1] 陈春妹[2] 郑煜芳[3] 徐丛剑[1] 

机构地区：[1]复旦大学附属妇产科医院妇产科,上海200011 [2]复旦大学遗传工程国家重点实验室 [3]复旦大学生命科学学院生物物理系

出　　处：《中华妇产科杂志》2010年第4期292-297,共6页Chinese Journal of Obstetrics and Gynecology

基　　金：国家自然科学基金（30700902）;上海市青年科技启明星计划（08QA1401600）

摘　　要：目的 研究piggyBac（PB）转座子介导转移外源基因HSV-tk在多种妇科恶性肿瘤细胞中的表达情况,探讨其作为一种可整合的非病毒载体在肿瘤基因治疗中的应用价值.方法 通过PCR技术扩增HSV-tk基因的编码区,定向克隆至PB表达载体PB[Act-RFP]DS,经酶切、测序鉴定为重组载体PB[Act-RFP,HSV-tk]DS（pPB/TK）.联合3种小同的转染试剂FuGENE HD、jetPEI及lipofectamine 2000,分别将pPB/TK转染入4种常见的妇科恶性肿瘤细胞株HeLa、JEG-3、SKOV3和HEC-1B.转染后以mRFP1为报告基因,经荧光显微镜观察和流式细胞仪分析转染效率;逆转录（RT）-PCR技术检测HSV-tk和mRFP1基因的表达;四甲基偶氮唑蓝实验测定不同浓度的更昔洛韦（GCV）对转染后细胞的杀伤作用.转染后细胞经流式细胞仪分选,极限稀释单克隆培养建立稳定转染株,并以反向PCR技术确定转座子插入基因组的位点.结果 （1）成功构建重组载体pPB/TK.（2）在3种转染试剂的辅助下,pPB/TK均可有效转染入HeLa、HEC-1B、SKOV3和JEG-3细胞;不同转染试剂辅助下pPB/TK在同种细胞中的转染效率各不相同,在HeLa细胞中,FuGENE HD的转染效率[（78.7±9.2）%]高于lipofectamine 2000[（54.1±11.4）%]和jetPEI][（46.5±7.4）%],分别比较,差异均有统计学意义（P〈0.05）;同一转染试剂辅助下pPB/TK在不同细胞中的转染效率也不相同,以FuGENE HD为转染试剂,pPB/TK在HeLa、JEG-3和SKOV3细胞中的转染效率分别为（78.7 ±9.2）%、（74.4±8.9）%和（83.2±9.7）%,高于HEC-1B细胞的（39.5±8.7）%,分别比较,差异均有统计学意义（P〈0.05）.（3）RT-PCR结果显示,4种细胞均有HSV-tk和mRFP1基因mRNA的表达.（4）GCV对转染有pPB/TK的HeLa、JEG-3、SKOV3和HEC-1B细胞的半数抑制浓度分别为1.29、3.35、0.09和13.28 μg/ml.10μg/ml GCV对转染有pPB/TK的SKOV3细胞抑制率高于单独转染pORF-HSVtk者,细胞抑制率分别为（86±9）%和（52±12）%,两者比较,差异有�Objective To investigate the expression of exogenous gene transferred by piggyBac （PB） transposon in various gynecological malignant cell lines and reveal its potential application of gene therapy in gynecological cancer.Methods Amplified herpes simplex virus thymidine kinase （HSV-tk） gene coding region by PCR and integrated it into PB expression vector, PB[Act-RFP]DS, for reconstructing PB[Act-RFP, HSV-tk]DS （pPB/TK）.By using different transfection reagents： FuGENE HD, jetPEI, lipofectamine 2000, pPB/TK together with helper plasmid Act-PBase were cotransfected into four mostly common gynecological malignant tumor cell lines HeLa, JEG-3, SKOV3 and HEC-1B.The mRFP1 report gene expressions was observed and detected by fluorescence microscope and flow cytometry to analyze transfection efficiency.The expressions of HSV-tk and mRFP1 gene were detected by reverse transcription PCR （RT-PCR）.The cytotoxic effect of various concentration of pro-drug ganciclovir （GCV） for transfected cells was detected by methyl thiazole tetrazolium assay.The transfected cells were positive sorted by flow cytometry and limiting diluted to obtain the stable transfected cell line.The insertion sites of foreign gene tranferred by PB transposon in genome were analyzed by inverse PCR.Results （1） Double digests analysis and sequences test demonstrated that pPB/TK vector was reconstructed successfully.（2） Using three different transfective reagents, PB trausposon transferred HSV-tk gene and mRFP1 gene into HeLa, HEC-1 B, SKOV3 and JEG-3 cell efficiently, and the transfection efficiency of pPB/TK for the same cell was different by using different transfective reagents; in Hela cell, the transfection efficiency of FuGENE HD [（78.7 ± 9.2） %]was higher than that of lipofectamine 2000 [（54.1 ± 11.4） %]and jetPEI [（46.5 ± 7.4） %, all P 〈 0.05] ; using the same transfective reagent, the transfection efficiency of pPB/TK was also different on various cell lines, using FuGENE HD, the transfeetion efficiency o

关 键 词：生殖器肿瘤 女(雌)性 DNA可移植因子 转染 转基因 单纯疱疹病毒属 胸苷激酶 发光蛋白质类 

分 类 号：R737.3[医药卫生—肿瘤]