Double suicide genes driven by kinase domain insert containing receptor promoter selectively kill human lung cancer cells.

Genetic Vaccines and Therapy Pub Date : 2011-03-22 DOI:10.1186/1479-0556-9-6

Junrong Ma, Mi Li, Longyong Mei, Qinghua Zhou, Lunxu Liu, Xijie Yu, Guowei Che

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引用次数: 7

Abstract

Background: To investigate the selective killing efficacy of the double suicide genes driven by KDR promoter.

Materials and methods: A double suicide gene system with the KDR promoter, pcDNA3-KDRp-CDglyTK, was constructed and transfected into lung cancer cell lines L9981 and NL9980, and human hepatocellular carcinoma cell line HepG2. The efficiency and specificity of the double suicide gene system were assayed by in vitro cellular proliferation and apoptosis, as well as in vivo xenograft studies.

Results: The transgenic CD and TK genes were only expressed in L9981 and NL9980 but not in HepG2 cells. Pre-treating transfected cells with 5-Fc and GCV significantly reduced proliferation, enhanced apoptosis in L9981 and NL9980 but not in HepG2 cells. The tumor formed by L9981 and NL9980 cells with the double suicide gene system was much smaller in vivo.

Conclusion: Tumor targeted expression of CDglyTK gene driven by KDR promotor represents a novel strategy for effective gene therapy of tumor with intrinsic KDR.

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含有受体启动子的激酶结构域插入片段驱动双自杀基因选择性杀伤人肺癌细胞。

背景:研究KDR启动子驱动的双自杀基因的选择性杀伤效果。材料与方法:构建含有KDR启动子pcDNA3-KDRp-CDglyTK的双自杀基因体系，转染肺癌细胞株L9981、NL9980和人肝癌细胞株HepG2。双自杀基因系统的效率和特异性通过体外细胞增殖和凋亡以及体内异种移植研究进行了检测。结果:转CD和TK基因仅在L9981和NL9980细胞中表达，在HepG2细胞中不表达。用5-Fc和GCV预处理转染细胞可显著降低L9981和NL9980细胞的增殖，增强细胞凋亡，但对HepG2细胞无明显影响。具有双自杀基因系统的L9981和NL9980细胞在体内形成的肿瘤要小得多。结论:KDR启动子驱动CDglyTK基因的肿瘤靶向表达是一种有效治疗内源性KDR肿瘤的新策略。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Genetic Vaccines and Therapy

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