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作 者:高峰[1] 温晓岩[1] 刘希江[1] 卜慧莲[1] 曹菲[1] 田学愎[1] 杨辉[1] 王鹏[1] 田玉科[1]
机构地区:[1]华中科技大学同济医学院附属同济医院麻醉学教研室,430030
出 处:《中华麻醉学杂志》2011年第9期1096-1098,共3页Chinese Journal of Anesthesiology
基 金:国家自然科学基垒(30700783,30901396);高等学校博士学科点专项科研基金新教师项目(20070487117);贝朗麻醉科学研究基金(2007)
摘 要:目的构建共表达抗基因RNA与铁蛋白基因的双启动子慢病毒载体。方法将铁蛋白重链基因构建人线性化的慢病毒载体pGC-FU,以获得中间质粒DGC-U-HF;进而将具有基因沉默效应的β-arrestin2抗基因RNA构建人中间质粒,以获得目的质粒pGC-agRNA-HF;通过病毒的包装和浓缩,应用RealtimePCR法检测重组慢病毒的滴度,应用NGl08-15细胞,采用Western blot和实时定量PCR检测抗基因RNA的基因沉默效应和铁蛋白的表达。结果抗基因RNA与铁蛋白均成功构建入慢病毒表达载体,病毒滴度2.00×109TU/ml,该病毒转染NGl08.15细胞后,β-arrestin2表达下调,铁蛋白表达上调。结论成功构建了表达抗基因RNA与铁蛋白基因的双启动子慢病毒载体。Objective To construct lentivirus vector expressing antigene RNA and ferritin gene.Methods Intermediate plasmid pGC-FU-HF was constructed by transfecting lentivirus vector pGC-FU with heavy chain ferritin subunit gene. The target plasmid pGC-agRNA-HF was subsequently constructed by transfecting the intermediate plasmid with β-arrestin 2 antigene RNA. The NG108-15 cells were transfected with the target plasmid. The titre of lentivirus vector was measured by RT-PCR. The expression of antigene RNA and ferritin gene was determined by Western blot and RT-PCR. Results Lentivirus vector was successfully transfected with antigene RNA and ferritin gene. The titre of lentivirus vector was 2.00 × 109 TU/ml. The expression of β-arrestin2 protein was down-regulated and the expression of ferritin protein up-regulated in the NG108-15 cells after being transfected with the lentivirus vector. Conclusion Lentivirus vector expressing antigene RNA and ferritin gene has been successfully constructed.
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