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作 者:李小权[1] 张树林[1] 成军[2] 王琦[2] 李国力[2] 洪源[2]
机构地区:[1]西安交通大学医学院第一附属医院儿科,陕西西安710061 [2]北京地坛医院传染病研究所,北京100011
出 处:《第四军医大学学报》2008年第16期1468-1471,共4页Journal of the Fourth Military Medical University
基 金:国家自然科学基金(30371288);国家重点基础研究项目(2004CB518908)
摘 要:目的:使用哺乳动物双杂交系统探讨HCV-core与HCBP12在人肝癌细胞HepG2细胞中的相互作用.方法:PCR分别扩增含HCV core及HCBP12的cDNA片段,克隆入pGEM-T载体,经测序正确后再分别克隆入哺乳动物双杂交的表达质粒PBIND和PACT中,并转染HepG2细胞,48h后检测细胞中报告基因luciferase activity的表达水平.结果:Dual-Luciferase Activety系统检测显示PBIND-core与PACT-HCBP12实验组萤火虫荧光与海肾素荧光的比值明显高于其他阴性对照组,但低于阳性对照组.结论:哺乳动物双杂交系统证实HCV核心蛋白与其结合蛋白HCBP12在人肝癌细胞系中HepG2中有一定的相互作用,为进一步研究HCV-core和HCBP12的功能奠定基础.AIM: To analyze the interaction between HCV core protein and HCBP12 in HepG2 cells using MammalianTM Two-Hybrid System. METHODS: cDNA fragments encoding HCV core protein and HCBP12 were respectively amplified by PCR and subsequently cloned into pGEM-T vector. Mter verified by sequencing, they were subcloned into two hybrid plasmids, PBIND and PACT. Then, PBIND-core, PACT-HCBP12 and pGSluc, a reporter vector, all were co-transfected into HepG2 cells. After 48 hours, the interaction between HCV core protein and HCBP12 was assayed by measuring reporter gene expression. RESULTS: Dual-lucfferase Reporter Assay showed that the lucfferase activity of the co-transfecfion experiment group was higher than that of the other negative control groups and lower than that of the positive control group. CONCLUSION: Mammalian Two-Hybrid Assay confirmed that HCBP12 can bind with HCV core protein to some extent, which lays foundation for further study on function of HCBP12 and HCV-core.
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