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用于靶向癌症治疗的人端粒酶逆转录酶启动子的克隆

[Cloning of human telomerase reverse transcriptase promoter for targeted cancer therapy].

作者信息

Li Fan, Tan Xiao-Hua, Peng Xiao-Jun, Cai Hong-Bing, Hu Da-Rong

机构信息

Institute of Liver Diseases, General Hospital of Bejing Command, Beijing 100700, China.

出版信息

Di Yi Jun Yi Da Xue Xue Bao. 2005 Feb;25(2):207-11.

PMID:15699008
Abstract

OBJECTIVE

An human telomerase reverse transcriptase (hTERT) promoter was cloned to investigate the effect of simplex virus-thymidine kinase (HSV-tk) gene-ganciclovir (GCV) system under control of this promoter on lung cancer cells A549.

METHODS

Specific primers were designed to amplify the core hTERT promoter from HepG2 genome. A set of expression vectors encoding LacZ or tk gene under control of hTERT or hCMV promoter was constructed through standard molecular cloning methods. After the transfection with lipofectamine 2000, reverse transcriptional PCR (RT-PCR) and beta-Gal staining were performed to examine the activity of the hTERT promoter. The cytotoxic effects of GCV/tk on A549 and MRC5 cells transfected with the plasmids encoding tk gene were evaluated by MTT assay.

RESULTS

The hTERT promoter containing -208-+40 bp of the upstream sequence of human telomerase was successfully cloned. beta-Gal staining and RT-PCR were used to detect the expression of Lac Z and the transcription of tk gene under control of the hTERT promoter, respectively, in A549 rather than MRC5 cells. Cyototoxic effect of GCV was observed only in the A549 but not MRC5 cells after the transfection with pDC511 hTERT/tk, and the effect was dose-dependent. The effect, however, was observed in cells transfected with pDC518 hCMV/tk.

CONCLUSION

The hTERT promoter cloned in this study can specifically control the target gene expression in telomerase-positive tumor cells but not the normal cells, suggesting that the HSV-tk/GCV system under control of the hTERT promoter is a promising targeted gene therapy for malignant tumors.

摘要

目的

克隆人端粒酶逆转录酶(hTERT)启动子,以研究该启动子调控下的单纯疱疹病毒胸苷激酶(HSV-tk)基因-更昔洛韦(GCV)系统对肺癌细胞A549的作用。

方法

设计特异性引物从HepG2基因组中扩增hTERT核心启动子。通过标准分子克隆方法构建一组在hTERT或hCMV启动子调控下编码LacZ或tk基因的表达载体。用脂质体2000转染后,进行逆转录聚合酶链反应(RT-PCR)和β-半乳糖苷酶染色以检测hTERT启动子的活性。通过MTT法评估GCV/tk对转染了编码tk基因质粒的A549和MRC5细胞的细胞毒性作用。

结果

成功克隆了包含人端粒酶上游序列-208- +40 bp的hTERT启动子。β-半乳糖苷酶染色和RT-PCR分别用于检测A549细胞而非MRC5细胞中hTERT启动子调控下LacZ的表达和tk基因的转录。用pDC511 hTERT/tk转染后,仅在A549细胞而非MRC5细胞中观察到GCV的细胞毒性作用,且该作用呈剂量依赖性。然而,在用pDC518 hCMV/tk转染的细胞中也观察到了该作用。

结论

本研究克隆的hTERT启动子可特异性调控端粒酶阳性肿瘤细胞而非正常细胞中的靶基因表达,提示hTERT启动子调控下的HSV-tk/GCV系统是一种有前景的恶性肿瘤靶向基因治疗方法。

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