通过Tet-On调控在SCID小鼠模型中对人乳腺癌进行自杀基因治疗。

Suicide gene therapy of human breast cancer in SCID mice model by the regulation of Tet-On.

作者信息

Hu Wei-xin, Zeng Zhao-jun, Luo Sai-qun, Chen Qian

机构信息

Molecular Biology Research Center, Xiangya Medical College, Central South University, Changsha 410078, China.

出版信息

Chin Med J (Engl). 2004 Mar;117(3):434-9.

PMID:15043787

Abstract

BACKGROUND

RevTet-On gene expression system was used to deliver the suicide gene tk to human breast cancer cell line MCF-7 and control the tk gene expression level. The animal model of human breast cancer on severe combined immune deficiency (SCID) mice was set up to explore the suicide gene therapy by the regulation of Tet-On.

METHODS

Herpes simplex virus-thymidine kinase (HSVtk) gene was inserted into the plasmid pRevTRE and the recombinant retroviral vector pRevTRE/HSVtk was constructed. Using modified calcium phosphate co-precipitation method, two transfections, pRevTRE/HSVtk and pRevTet-On were performed for MCF-7 cell line and selected by hygromycin B and G418. MCF-7 cell line that stably expressed Tet-regulated tk gene was established. HSVtk gene expression in the MCF/TRE/tk/Tet-On cell line was under the control of Doxycycline (Dox). Cell viability was also determined by MTT assay, whereas HSVtk gene expression was analyzed by reverse transcription-PCR (RT-PCR).

RESULTS

MCF/TRE/tk/Tet-On cell survival rate was decreased from 100% to less than 20% when ganciclovir (GCV) concentration was increased from 0 to 1000 microg/ml at 1 microg/ml of Dox after 72 hours of GCV administration. At 1 microg/ml of GCV concentration, the cell numbers decreased from 7 x 10(4) cells/ml to 2 x 10(4) cells/ml when Dox concentration was increased from 0 to 1500 ng/ml after 72 hours culture. In addition, bystander effects were generated in vitro when 10% - 25% of transduced MCF-7 cells were mixed in untransduced MCF-7 cells. On the other hand, the human breast cancer models in SCID mice were set up. The tk gene was expressed with the regulated character after MCF/TRE/tk/Tet-On cells were implanted into the female SCID mice 7 days after Dox induction followed by intraperitoneally administration of GCV for 23 days. Subcutaneous tumors in SCID mice that were implanted with MCF/TRE/tk/Tet-On cells shrank remarkably after Dox and GCV administration as compared with the control.

CONCLUSION

The human breast tumor cells (MCF-7) expressing HSVtk gene can be eradicated by administration of GCV and induced with tetracycline or its derivative Dox in vitro and in vivo.

摘要

背景

采用RevTet-On基因表达系统将自杀基因tk导入人乳腺癌细胞系MCF-7，并调控tk基因的表达水平。建立重度联合免疫缺陷（SCID）小鼠人乳腺癌动物模型，以探索通过Tet-On调控进行自杀基因治疗。

方法

将单纯疱疹病毒胸苷激酶（HSVtk）基因插入质粒pRevTRE，构建重组逆转录病毒载体pRevTRE/HSVtk。采用改良磷酸钙共沉淀法，对MCF-7细胞系进行pRevTRE/HSVtk和pRevTet-On两次转染，并用潮霉素B和G418进行筛选。建立稳定表达Tet调控tk基因的MCF-7细胞系。MCF/TRE/tk/Tet-On细胞系中HSVtk基因的表达受强力霉素（Dox）调控。通过MTT法测定细胞活力，采用逆转录聚合酶链反应（RT-PCR）分析HSVtk基因表达。

结果

在1μg/ml Dox存在下，给予更昔洛韦（GCV）72小时后，当GCV浓度从0增加到1000μg/ml时，MCF/TRE/tk/Tet-On细胞存活率从100%降至20%以下。在1μg/ml GCV浓度下，培养72小时后，当Dox浓度从0增加到1500ng/ml时，细胞数量从7×10⁴个细胞/ml降至2×10⁴个细胞/ml。此外，当10% - 25%转导的MCF-7细胞与未转导的MCF-7细胞混合时，在体外产生了旁观者效应。另一方面，建立了SCID小鼠人乳腺癌模型。在Dox诱导7天后，将MCF/TRE/tk/Tet-On细胞植入雌性SCID小鼠体内，随后腹腔注射GCV 23天，tk基因呈调控性表达。与对照组相比，给予Dox和GCV后，植入MCF/TRE/tk/Tet-On细胞的SCID小鼠皮下肿瘤明显缩小。