人p27~(kipl)可调控性重组腺病毒载体的构建及其在PC-3细胞中的表达 Construction of regulatory human p27~kipl recombinant adenovirus vector and its expression in human prostate cancer cell line PC-3期刊界 All Journals 搜尽天下杂志传播学术成果专业期刊搜索期刊信息化学术搜索

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人p27~(kipl)可调控性重组腺病毒载体的构建及其在PC-3细胞中的表达

引用本文：	邱镇,孙颖浩,许传亮,王元天,沈茜,钱松溪,顾正勤,李云,Chinlee Wu.人p27~(kipl)可调控性重组腺病毒载体的构建及其在PC-3细胞中的表达[J].第二军医大学学报,2003,24(11):1200-1203.

作者姓名：	邱镇孙颖浩许传亮王元天沈茜钱松溪顾正勤李云 Chinlee Wu

作者单位：	第二军医大学长海医院泌尿外科,第二军医大学长海医院泌尿外科,第二军医大学长海医院泌尿外科,第二军医大学长海医院泌尿外科,长海医院中心实验室,第二军医大学长海医院泌尿外科,第二军医大学长海医院泌尿外科,第二军医大学长海医院泌尿外科,Department of Pathology,Massachusetts General Hospital,Bigelow 1102,55 Fruit Street,Boston,MA 2114-2696,USA 上海200433,上海200433,上海200433,上海200433,上海200433,上海200433,上海200433

基金项目：	国家自然科学基金重大国际合作研究项目(30110665),全军医药科研“十五”规划重点课题(012067)

摘要：	目的:体外构建人p27kipl可调控性重组腺病毒载体,并观察其在前列腺癌细胞系PC-3细胞中的表达及其对细胞生长的影响。方法:采用Ad-X Tet-Off表达系统,将人全长p27kipl cDNA经过穿梭载体,与可调控性腺病毒载体骨架连接,得到重组人p27kipl基因腺病毒(Ad-p27kipl),在HEK293细胞包装、扩增,获得高滴度病毒,采用空斑试验测定病毒滴度,体外转染PC-3细胞,RT-PCR、Western杂交分别检测目的基因不同水平的表达,并通过MTT法观察转染前后细胞增殖力的变化。Ad-X-TRE-β gal病毒作为对照。结果:构建的Ad-p27kipl病毒滴度为1.2×109 pfu/ml,RT-PCR、Western杂交检测有特异的高表达,转染后对细胞的生长有抑制作用。结论:体外连接法成功地构建携带人p27kipl基因的可调控性重组腺病毒载体,在人前列腺癌细胞系PC-3中有高表达并对细胞生长有抑制作用。
关键词：	前列腺癌 p27kipl 腺病毒载体 PC-3细胞株
Construction of regulatory human p27~kipl recombinant adenovirus vector and its expression in human prostate cancer cell line PC-3

QIU Zhen,SUN Ying-Hao,XU Chuan-Liang,WANG Yuan-Tian,SHEN Qian,QIAN Song-Xi,GU Zheng-Qin,Yun,Chinlee Wu.Construction of regulatory human p27~kipl recombinant adenovirus vector and its expression in human prostate cancer cell line PC-3[J].Academic Journal of Second Military Medical University,2003,24(11):1200-1203.

Authors:	QIU Zhen SUN Ying-Hao XU Chuan-Liang WANG Yuan-Tian SHEN Qian QIAN Song-Xi GU Zheng-Qin Yun Chinlee Wu

Abstract:	Objective:To construct regulatory human p27kipl recombinant adenovirus vector and analyze its expression in human prostate cancer cell line PC-3 and its effects on cell proliferation. Methods: The full-length cDNA encoding p27*"v] gene was inserted into pTRE-Shuttle vector. Then the expression cassette containing tetracycline-responsive element, which regulating the expression of inserted genes, was excised with restriction enzymes PI-Sce I and I-Ceu I and ligated to the backbone of the Adeno-X viral DNA. The recombinant adenovirus plasmid was identified by restriction enzymes excising analysis and PCR. The replication-incompetent recombinant adenovirus was packaged and propagated in HEK293 cells. The viral titer was examined by plaque assay; the mRNA and protein expressions of p27kipl were determined by RT-PCR and Western bolt respectively. MTT assay was used to assess the effect of p27kipl on cell proliferation. Ad-X-TRE (3 gal virus was used as control. Results: The viral liter of Ad-p27kipl was 1. 2X 109 pfu/ml and the P27 protein expression was positive and high. The growth of PC-3 cells treated with Ad-p27kipl was significanlly inhibiled compared with that treated with control adenovirus. Conclusion; The human p27kipl recombinanl adenovirus has been successfully built and is highly expressed in human prostate cancer cell line PC-3. Adenoviral-mediated expression of human p27kipl can inhibit the proliferation of human proslate cancer cell lines PC-3.

Keywords:	prostate cancer p27kipl adenovirus vector PC-3 cell line
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