肿瘤研究与临床
腫瘤研究與臨床
종류연구여림상
CANCER RESEARCH AND CLINIC
2011年
4期
220-222
,共3页
董伦%韩崇旭%宿建辉%李健%张恒柱%张宪%佘磊%武永康
董倫%韓崇旭%宿建輝%李健%張恆柱%張憲%佘磊%武永康
동륜%한숭욱%숙건휘%리건%장항주%장헌%사뢰%무영강
微RNA-7-3%慢病毒载体%绿色荧光蛋白质%神经胶质瘤
微RNA-7-3%慢病毒載體%綠色熒光蛋白質%神經膠質瘤
미RNA-7-3%만병독재체%록색형광단백질%신경효질류
MicroRNA-7-3%Lentiviral vector%,Green fluorescent protein%Gliomas
目的 构建人类mir-7-3基因慢病毒表达载体,为进一步研究mir-7-3基因的功能及其在肿瘤治疗中的应用奠定基础.方法 采用反转录-聚合酶链(RT-PCR)技术从含有mir-7-3基因的质粒pENTR-MIRNA VECTOR扩增目的 基因mir-7-3,并将基因克隆到慢病毒载体表达质粒Lenti-GFP-RNAiVECTOR[含增强型绿色荧光蛋白(EGFP)基因]中,构建慢病毒载体表达质粒Lenti-GFP-mir-7-3,酶切、测序验证mir-7-3基因后,将Lenti-GFP-mir-7-3质粒和包装质粒pRsv-REV、pMDlg-pRRE、pMD2G共同转染人类胚胎肾上皮细胞系293T细胞,获得携带mir-7-3基因和EGFP基因的重组慢病毒FIV-CMV-EGFP-mir-7-3,取浓缩纯化后的病毒上清感染293T细胞和人类胶质瘤细胞U251,荧光显微镜观察293T细胞的荧光表达,RT-PCR鉴定U251细胞中mir-7-3基因的表达水平.结果 Lenti-GFP-mir-7-3共转染包装细胞293T能产生高浓度的重组慢病毒FTV-CMV-EGFP-mir-7-3,荧光显微镜下能直接观察到EGFP,FIV-CMV-EGFP-mir-7-3中携有正确的mir-7-3基因,目的 基因mir-7-3能被重组慢病毒高效地转导人U251.结论 成功构建了携带mir-7-3基因的重组慢病毒载体;为进一步从分子水平探讨mir-7-3基因治疗胶质瘤奠定了基础.
目的 構建人類mir-7-3基因慢病毒錶達載體,為進一步研究mir-7-3基因的功能及其在腫瘤治療中的應用奠定基礎.方法 採用反轉錄-聚閤酶鏈(RT-PCR)技術從含有mir-7-3基因的質粒pENTR-MIRNA VECTOR擴增目的 基因mir-7-3,併將基因剋隆到慢病毒載體錶達質粒Lenti-GFP-RNAiVECTOR[含增彊型綠色熒光蛋白(EGFP)基因]中,構建慢病毒載體錶達質粒Lenti-GFP-mir-7-3,酶切、測序驗證mir-7-3基因後,將Lenti-GFP-mir-7-3質粒和包裝質粒pRsv-REV、pMDlg-pRRE、pMD2G共同轉染人類胚胎腎上皮細胞繫293T細胞,穫得攜帶mir-7-3基因和EGFP基因的重組慢病毒FIV-CMV-EGFP-mir-7-3,取濃縮純化後的病毒上清感染293T細胞和人類膠質瘤細胞U251,熒光顯微鏡觀察293T細胞的熒光錶達,RT-PCR鑒定U251細胞中mir-7-3基因的錶達水平.結果 Lenti-GFP-mir-7-3共轉染包裝細胞293T能產生高濃度的重組慢病毒FTV-CMV-EGFP-mir-7-3,熒光顯微鏡下能直接觀察到EGFP,FIV-CMV-EGFP-mir-7-3中攜有正確的mir-7-3基因,目的 基因mir-7-3能被重組慢病毒高效地轉導人U251.結論 成功構建瞭攜帶mir-7-3基因的重組慢病毒載體;為進一步從分子水平探討mir-7-3基因治療膠質瘤奠定瞭基礎.
목적 구건인류mir-7-3기인만병독표체재체,위진일보연구mir-7-3기인적공능급기재종류치료중적응용전정기출.방법 채용반전록-취합매련(RT-PCR)기술종함유mir-7-3기인적질립pENTR-MIRNA VECTOR확증목적 기인mir-7-3,병장기인극륭도만병독재체표체질립Lenti-GFP-RNAiVECTOR[함증강형록색형광단백(EGFP)기인]중,구건만병독재체표체질립Lenti-GFP-mir-7-3,매절、측서험증mir-7-3기인후,장Lenti-GFP-mir-7-3질립화포장질립pRsv-REV、pMDlg-pRRE、pMD2G공동전염인류배태신상피세포계293T세포,획득휴대mir-7-3기인화EGFP기인적중조만병독FIV-CMV-EGFP-mir-7-3,취농축순화후적병독상청감염293T세포화인류효질류세포U251,형광현미경관찰293T세포적형광표체,RT-PCR감정U251세포중mir-7-3기인적표체수평.결과 Lenti-GFP-mir-7-3공전염포장세포293T능산생고농도적중조만병독FTV-CMV-EGFP-mir-7-3,형광현미경하능직접관찰도EGFP,FIV-CMV-EGFP-mir-7-3중휴유정학적mir-7-3기인,목적 기인mir-7-3능피중조만병독고효지전도인U251.결론 성공구건료휴대mir-7-3기인적중조만병독재체;위진일보종분자수평탐토mir-7-3기인치료효질류전정료기출.
Objective To construct a lentiviral vector containing mir-7-3 gene and green fluorescent protein (GFP) gene,and to detect the expression of mir-7-3 gene in U251 cells.Methods The fragments containing all the mir-7-3 gene were amplified by RT-PCR and were cloned into the lentivirus vectors labeled with GFP,which was transfected together with the packaging plasmids into 293T cells by CaC12.The supernatant was collected,concentrated,identified,and was transfected to U251 cells of gliomas.Fluorescent microscopy was used to observe the fluorescence in the 293T cell,and real time RT-PCR was used to examine the relative contents of mir-7-3 in U251 cells.Results Electrophores was shown that the sequence of the RT-PCR product was consistent with the data of mir-7-3 by DNA sequence analysis,indicating that the mir-7-3 gene was successfully cloned,and strong green fluorescence was observed by fluorescent microscopy.The supernatant of lentivirus-transfected 293T cells effectively infected U251 cells and the relative content of mir-7-3 was observed in the transfected U251 cells.Conclusion It is concluded that the lentiviral vector containing mir-7-3 gene was constructed successfully,which provides a basis for further study of mir-7-3 function.
