Please wait a minute...
浙江大学学报(医学版)
浙江大学学报(医学版)  2014, Vol. 43 Issue (2): 193-199    DOI: 10.3785/j.issn.1008-9292.2014.03.013
论著     
整合素连接激酶基因敲降和黑色素瘤分化相关基因过表达慢病毒载体构建和鉴定
杨幼萍1,丁燕2,王继荣3,曾玲晖3,林红霞1,朱杨丽1,吴宏卫1,王若燕1,张建民1,应荣彪1
1. 浙江省台州市肿瘤医院,浙江 温岭 310075
2. 台州市中心医院,浙江 台州 318000
3. 浙江大学城市学院医学院,浙江 杭州 310015
Construction and identification of lentiviral vector containing human ILK-shRNA and mda7 gene
YANG You-ping 1, DING Yan2, WANG Ji-rong2, ZENG Ling-hui2, LIN Hong-xia1, ZHU Yang-li1, WU Hong-wei1, WANG Ruo-yan1, ZHANG Jian-min1, YING Rong-biao1
1.Taizhou Cancer Hospital, Wenling 310075, China; 2.Taizhou Central Hospital, Taizhou 318000, China; 3. Zhejiang University City College, School of Medicine, Hangzhou 310015, China
全文: PDF(958 KB)  
摘要: 

目的:建立整合素相关激酶(ILK)基因敲降和黑色素瘤分化相关基因(mda7)过表达慢病毒包装表达系统。方法:针对人ILK基因序列,设计基因敲降靶点序列(A、B、C),通过限制性内切酶HpaⅠ和XhoⅠ双酶切、T4 DNA连接酶连接,将ILK插入慢病毒载体pSicoR-eGFP,构建siILK-pSicoR-eGFP重组质粒;根据人mda7基因序列,设计引物扩增mda7全长,并插入慢病毒载体pLVX-Puro,构建mda7-pLVX-Puro重组质粒。经双酶切及测序鉴定正确后通过脂质体将慢病毒四质粒系统共转染人胚肾细胞系293T细胞,进行慢病毒包装并测定病毒滴度、观察感染效率。各组病毒载体转染PC-3细胞后,用定量PCR和蛋白质印迹法检测ILK基因和mda7 mRNA转录水平及蛋白表达水平。通过MTT法和Transwell实验考察ILK和mda7对PC-3细胞增殖和迁移的影响。结果:成功构建ILK基因敲降及mda7过表达的慢病毒载体,四质粒系统共转染293T细胞后可见大量绿色荧光染色阳性细胞。浓缩病毒后293T细胞的感染效率在90%以上,并能高效率感染PC-3前列腺癌细胞。ILK-A-pSicoR-eGFP和ILK-B-pSicoR-eGFP组ILK干扰效果最佳(P<0.05),mda7的表达水平远高于对照组(P<0.05),且持续稳定表达至少1个月。ILK和mda7对PC-3细胞的增殖在96 h内有明显抑制作用,并对其迁移亦有显著抑制(均P<0.05)。结论:成功构建并鉴定人ILK 基因敲降和mda7过表达慢病毒载体,可为探讨ILK和mda7基因在肿瘤细胞中的生物学功能提供良好工具,也为探索安全、高效的肿瘤治疗途径奠定实验基础。
关键词 整合素类磷酸转移酶类前列腺肿瘤白细胞介素类基因 肿瘤抑制慢病毒属/遗传学遗传载体基因表达    
Abstract

Objective: To construct and identify lentiviral vector containing human ILK-shRNA and mda7 gene.Methods: Based on the human ILK gene sequences, RNAi target sequences were designed and cloned into the lentiviral vector pSicoR-eGFP by restriction endonuclease HpaⅠ and XhoⅠ double digestion and T4 DNA ligase ligation. Based on the human mda7 gene sequences, PCR primers were designed to clone the full-length mda7, and were cloned into the lentiviral vector pLVX-Puro. After the candidate clones were identified by DNA sequencing, the recombinant plasmid and the three packaging plasmids were co-transfected into the human embryonic kidney 293T cells by lipofectamine 2000 to produce the lentiviral particles. Human prostate cancer PC-3 cells were infected with the constructed lentiviral vector. The ILK and mda7 expression levels in PC-3 cells were quantified by qPCR and Western blot, respectively. The effect of ILK and mda7 on proliferation and migration of PC-3 cells were assessed by MTT method and Transwell assay, respectively.Results: ILK-pSicoR-eGFP and mda7-pLVX-Puro lentiviral vectors were successfully constructed. Strong green fluorescence was observed in the 293T cells under the fluorescent microscope after co-transfection of 293T cells with 4 plasmids of lentiviral vector. The transfection efficiency of the collected virus exceeded 90% in the 293T cells and the PC-3 cells were infected with the lentiviral particles with high efficiency. The A and B lentiviral vector inhibited the expression of ILK at both the mRNA and protein levels in PC-3 cells significantly. The mda7-pLVX-Puro lentiviral vector increased the expression of mda7 in PC-3 cells, and the ability was maintained for one month. Within 96 h, ILK and mad7 significantly inhibited the proliferation and migration of PC-3 cells (Ps<0.05). Conclusion: The lentiviral vectors of ILK knockdown and mda7 over-expression have been successfully constructed and identified. The recombinant lentivirus can efficiently infect human prostate cancer PC-3 cells, in which ILK expression is inhibited and mda7 is over-expressed.
Key wordsIntegrins    Phosphotransferases    Prostatic neoplasms    Interleukins    Genes, tumor suppressor    Lentivirus/genetics    Genetic vectors    Gene expression
收稿日期: 2013-08-20     
基金资助:

浙江省自然科学基金(LY12H16005).
通讯作者: 应荣彪(1969-),男,学士,主任医师,从事临床肿瘤外科工作;E-mail: yingrongbiao@163.com   
Corresponding author: YING Rong-biao, E-mail: yingrongbiao@163.com   
作者简介: 杨幼萍(1960-),女,学士,主任医师,从事临床肿瘤外科工作;E-mail: yyp0576@163.con
服务  
把本文推荐给朋友
加入引用管理器
E-mail Alert
RSS
作者相关文章  
杨幼萍
丁燕
王继荣
曾玲晖
林红霞
朱杨丽
吴宏卫
王若燕
张建民
应荣彪

引用本文:

杨幼萍,丁燕,王继荣,曾玲晖,林红霞,朱杨丽,吴宏卫,王若燕,张建民,应荣彪. 整合素连接激酶基因敲降和黑色素瘤分化相关基因过表达慢病毒载体构建和鉴定[J]. 浙江大学学报(医学版), 2014, 43(2): 193-199.
YANG You-ping, DING Yan, WANG Ji-rong, ZENG Ling-hui, LIN Hong-xia, ZHU Yang-li, WU Hong-wei, WANG Ruo-yan, ZHANG Jian-min, YING Rong-biao. Construction and identification of lentiviral vector containing human ILK-shRNA and mda7 gene. Journal of ZheJiang University(Medical Science), 2014, 43(2): 193-199.

链接本文:

http://www.zjujournals.com/xueshu/med/CN/10.3785/j.issn.1008-9292.2014.03.013      或      http://www.zjujournals.com/xueshu/med/CN/Y2014/V43/I2/193

[1] 李统宇 等. 杜氏肌营养不良疾病模型及基因治疗研究进展[J]. 浙江大学学报(医学版), 2016, 45(6): 648-654.
[2] 方清清 等. 低频脉冲电磁场促进成骨细胞分化的基因调节和非基因调节探究[J]. 浙江大学学报(医学版), 2016, 45(6): 568-574.
[3] 候仕芳 等. 下调lmna基因对斑马鱼胚胎髓系和红系造血干细胞发育的影响[J]. 浙江大学学报(医学版), 2016, 45(6): 620-625.
[4] 吴志华 等. 异基因造血干细胞移植受者T细胞受体β链CDR3谱型表达与巨细胞病毒激活[J]. 浙江大学学报(医学版), 2016, 45(5): 515-521.
[5] 方敏波 等. 瞬时受体电位通道M2外显子单核苷酸多态性rs1556314与脓毒症的相关性分析[J]. 浙江大学学报(医学版), 2016, 45(4): 410-415.
[6] 娄鹏荣 等. 靶向RAD18的小干扰RNA对人食管鳞癌ECA-109细胞增殖和化疗敏感性的影响[J]. 浙江大学学报(医学版), 2016, 45(4): 364-370.
[7] 林伟仁 等. zeste基因增强子同源物2抑制剂GSK126对前列腺癌细胞的作用及机制[J]. 浙江大学学报(医学版), 2016, 45(4): 356-363.
[8] 陈晓静 等. 微RNA-let-7e-3p在宫颈上皮内瘤变和宫颈癌组织中的表达及临床意义[J]. 浙江大学学报(医学版), 2016, 45(4): 342-348.
[9] 沈志森 等. RNA干扰沉默DJ-1基因对Hep-2细胞裸鼠移植瘤生长的影响[J]. 浙江大学学报(医学版), 2016, 45(4): 349-355.
[10] 周琦惠 等. 人类免疫缺陷病毒储存库评估测定技术研究进展[J]. 浙江大学学报(医学版), 2016, 45(3): 256-260.
[11] 姜丽娇 等. 非全身型幼年特发性关节炎患儿外周血T辅助细胞1/2细胞因子水平分析[J]. 浙江大学学报(医学版), 2016, 45(3): 281-286.
[12] 王程 等. 微RNA:一类新的椎间盘退变调控因子[J]. 浙江大学学报(医学版), 2016, 45(2): 170-178.
[13] 何虹 等. 重组腺病毒载体介导外源性水通道蛋白基因经导管逆行注射治疗干燥综合征研究进展[J]. 浙江大学学报(医学版), 2016, 45(1): 86-90,97.
[14] 苏敏 等. 基于可变数目串联重复序列的痰液结核分枝杆菌检测方法建立及初步应用[J]. 浙江大学学报(医学版), 2016, 45(1): 61-67.
[15] 徐力等. SN-38与索拉非尼联合应用体外抗肝癌效果及其机制[J]. 浙江大学学报(医学版), 2015, 44(5): 486-492.