文章摘要
尹小菲 谭晓华 李靖 何敏 杨磊.vFLIP激活Jurkat细胞表达HIV 抑制因子的研究[J].,2015,15(23):4449-4452
vFLIP激活Jurkat细胞表达HIV 抑制因子的研究
vFLIP Stimulates Anti-HIV Factors Expression in Jurkat Cells
  
DOI:
中文关键词: KSHV  HIV抑制因子  vFLIP  Jurkat
英文关键词: KSHV  HIV Inhibitory Factors  vFLIP  Jurkat
基金项目:浙江省科技厅国际合作重点项目(2009C14014)
作者单位
尹小菲 谭晓华 李靖 何敏 杨磊 成都医学院生物医学系杭州师范大学医学院杭州师范大学生命与环境科学学院 
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中文摘要:
      目的:检测KSHV 编码的vFLIP 蛋白对Jurkat 细胞HIV 抑制因子表达的影响。方法:本研究首先构建真核表达载体 pIRES2-EGFP-vFLIP,再将其电穿孔至Jurkat 细胞,然后使用实时荧光定量PCR 技术检测Jurkat 细胞中A3G、A3F、CCL5 等HIV 抑制因子的表达水平,从而探讨vFLIP 抗HIV/AIDS 的作用及机制。结果:成功构建了真核表达载体pIRES2-EGFP-vFLIP,电转 染效率达到40%左右。与对照载体转染组相比,vFLIP转染组内Jurkat 细胞中CCL5、A3G、A3F 及Mx2 基因的表达分别上调了 6.71、2.20、1.52 及14.47 倍。结论:vFLIP 蛋白可以激活Jurkat细胞内某些HIV 抑制因子的表达,提示其具有一定的抗HIV/AIDS 作用。
英文摘要:
      Objective:To detect the effect of vFLIP on expression levels of anti-HIV factors in Jurkat cells.Methods:In this study, we constructed the eukaryotic expressive vector of pIRES2-EGFP-vFLIP and transfected the vector to Jurkat cells by electroporation. Then we detected the relative expression levels of anti-HIV factors in vFLIP transfected Jurkat cells by qPCR. Finally, we discussed the functions and mechanisms of vFLIP against HIV/AIDS.Results:The eukaryotic expressive vector of pIRES2-EGFP-vFLIP was successfully constructed. The transfection efficiency of vectors were about 40%. In comparison with pIRES2-EGFP transfected cells, the pIRES2-EGFP-vFLIP transfected cells can increase expression levels of CCL5, A3G, A3F and Mx2 in Jurkat cells by 6.71, 2.20, 1.52 and 14.47 times seperately.Conclusion:vFLIP can activate expressions of CCL5, A3G, A3F and Mx2 in Jurkat cells, and thus suggesting that vFLIP may have the function of anti-HIV/AIDS .
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