摘要
用 PCR方法扩增了鸡贫血病毒标准株的 vp3基因 ,并将其克隆于真核表达载体 pc DNA3上 ,构建了重组体pc DNA- vp3。经酶切鉴定及测序分析表明 ,该片段和预期相符。在体外利用 L ipofect AMINETM介导的基因转染 ,将 pc D-NA- vp3、 pc DNA3分别转入肝癌细胞系 Hep G2和二倍体肝细胞系 L- 0 2中 ,转染后的 RT- PCR结果证实 vp3基因在细胞中得到了表达。同时利用筛选稳定表达细胞株的技术和原位细胞凋亡检测法 ,证明了鸡贫血病毒是以凋亡的方式诱导细胞死亡 ,并且只诱导癌细胞的凋亡 ,而不诱导正常或二倍体细胞死亡。表明鸡贫血病毒
Using PCR technique, the vp3 gene of chicken anemia virus (CAV) was cloned into the eukaryotic expression vector pcDNA3 to construct a recombinant pcdNA vp3. Restriction enzyme and sequencing analysis revealed that CAV vp3 gene was correctly inserted into the blank vector pcDNA3. Total mRNA was extracted from liver carcinoma cell lines HepG2 and diploid cell line L 02 after LipofectAMINE TM mediated transfection in vitro with pcDNA vp3. After that, RT PCR was performed. The results of RT PCR suggested that vp3 gene was expressed in these two cell lines. At the same time, using in situ apoptotic detection assay, TUNEL Kits, the apoptotic cells were found in pcDNA vp3 transfected HepG2, but not in mock transfected cell lines. vp3 could induce cell death by apoptosis. vp3 could only induce apoptosis in cancer cell lines, but not in diploid cell lines. All the results indicated that CAV vp3 gene, a potential therapeutic agents, would be used widely in treating cancers in future
出处
《同济医科大学学报》
CAS
CSCD
北大核心
2001年第4期300-303,共4页
Acta Universitatis Medicinae Tongji
