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[靶向端粒酶RNA核酶的构建、筛选及端粒酶核酶对CNE-2Z细胞增殖和凋亡的影响]

[Construction and screening of a ribozyme targeting telomerase RNA and effects of telomerase ribozyme on proliferation and apoptosis of CNE-2Z cells].

作者信息

Zhao Ying-Hai, Chen Xiao-Yi, R Arrand John

机构信息

Department of Pathology, Guangdong Medical College, Zhanjiang, Guangdong, 524023, P.R.China.

出版信息

Ai Zheng. 2004 Jan;23(1):50-5.

PMID:14720374
Abstract

BACKGROUND & OBJECTIVE: It was proved that telomerase is an important determinant in tumor progression and cell immortalization. Ribozyme is a special kind of trans-acting RNA with endonuclease activity and sequence-specific catalytic RNA molecules, which can cleave target RNA. It was reported that telomerase activity is present in human poorly-differentiated nasopharyngeal carcinoma (NPC) CNE-2Z cells. This study was designed to construct eukaryotic expression plasmids containing telomerase ribozyme (teloRZ)gene targeting the template region of human telomerase RNA (hTR) and then to transfect the plasmids into CNE-2Z cells by electroporation to investigate the effect of teloRZ on proliferation and apoptosis of those transfected CNE-2Z cells.

METHODS

Hammer ribozyme gene teloRZ directed against telomerase RNA templet was designed and synthesized to serve as a telomerase inhibitor. Three different eukaryotic expression plasmids carried with the green fluorescent protein (GFP) reporter gene and puromycin-resistance gene and containing teloRZ gene were constructed. They were referred to as pGFPuro-teloRZ2.1, pGFPuro-teloRZ7.1, and pGFPuro-teloRZ7.7 and differed in the relative orientation of the genes for telomerase-ribozyme and puromycin-resistance. The CNE-2Z cells were transfected with three expression plasmids and control plasmid pPAT-GFP by electroporation. The expression of GFP was detected by fluorescent microscope; cellular proliferation index (PI) and apoptosis were investigated by flow cytometry analysis and fluorescence staining.

RESULTS

PI of CNE-2ZGTR7.1 cells transfected by plasmid pGFPuro-teloRZ7.1 (25.100%+/-0.141%)was significantly lower than those of CNE-2Z cells untransfected by any plasmid (53.663%+/-16.981%),CNE-2ZG cells transfected by control plasmid pPAT-GFP (61.575%+/-5.166%),CNE-2ZGTR2.1 cells transfected by plasmid pGFPuro-teloRZ2.1 (61.500%+/-20.082%), and CNE-2ZGTR7.7 cells transfected by plasmid pGFPuro-teloRZ7.7 (59.400%+/-13.933%) (P< 0.01). GFP was detected in CNE-2ZG cells,CNE-2ZGTR7.1 cells, and CNE-2ZGTR7.7 cells;while there was no GFP expression in CNE-2Z cells and CNE-2ZGTR2.1 cells. The plasmid pGFPuro-teloRZ7.1 was selected from 3 plasmids for further experiments. Apoptosis could be observed in CNE-2ZGTR7.1 cells after 12 generations. There was no apoptosis occurring in CNE-2Z and CNE-2ZG cells.

CONCLUSION

The teloRZ7.1 gene was electroporated successfully into CNE-2Z cells. TeloRZ7.1 can inhibit the proliferation and induce apoptosis of CNE-2Z cells. These findings suggest the potential application of ribozyme teloRZ7.1 as telomerase inhibitor.

摘要

背景与目的

已证实端粒酶是肿瘤进展和细胞永生化的重要决定因素。核酶是一类具有内切酶活性的特殊反式作用RNA和序列特异性催化RNA分子,可切割靶RNA。据报道,人低分化鼻咽癌(NPC)CNE-2Z细胞中存在端粒酶活性。本研究旨在构建针对人端粒酶RNA(hTR)模板区域的含端粒酶核酶(teloRZ)基因的真核表达质粒,然后通过电穿孔将质粒转染至CNE-2Z细胞,以研究teloRZ对转染的CNE-2Z细胞增殖和凋亡的影响。

方法

设计并合成针对端粒酶RNA模板的锤头状核酶基因teloRZ作为端粒酶抑制剂。构建了三种携带绿色荧光蛋白(GFP)报告基因和嘌呤霉素抗性基因且含有teloRZ基因的不同真核表达质粒。它们分别称为pGFPuro-teloRZ2.1、pGFPuro-teloRZ7.1和pGFPuro-teloRZ7.7,端粒酶核酶基因和嘌呤霉素抗性基因的相对方向不同。通过电穿孔将三种表达质粒和对照质粒pPAT-GFP转染至CNE-2Z细胞。用荧光显微镜检测GFP的表达;通过流式细胞术分析和荧光染色研究细胞增殖指数(PI)和凋亡情况。

结果

用质粒pGFPuro-teloRZ7.1转染的CNE-2ZGTR7.1细胞的PI(25.100%±0.141%)显著低于未转染任何质粒的CNE-2Z细胞(53.663%±16.981%)、用对照质粒pPAT-GFP转染的CNE-2ZG细胞(61.575%±5.166%)、用质粒pGFPuro-teloRZ2.1转染的CNE-2ZGTR2.1细胞(61.500%±20.082%)以及用质粒pGFPuro-teloRZ7.7转染的CNE-2ZGTR7.7细胞(59.400%±13.933%)(P<0.01)。在CNE-2ZG细胞、CNE-2ZGTR7.1细胞和CNE-2ZGTR7.7细胞中检测到GFP;而在CNE-2Z细胞和CNE-2ZGTR2.1细胞中未检测到GFP表达。从三种质粒中选择质粒pGFPuro-teloRZ7.1进行进一步实验。传代12代后,在CNE-2ZGTR7.1细胞中可观察到凋亡。在CNE-2Z和CNE-2ZG细胞中未发生凋亡。

结论

teloRZ7.1基因成功电穿孔导入CNE-2Z细胞。TeloRZ7.1可抑制CNE-2Z细胞的增殖并诱导其凋亡。这些发现提示核酶teloRZ7.1作为端粒酶抑制剂的潜在应用价值。

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