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A new generation of pPRIG-based retroviral vectors

机译:新一代基于pPRIG的逆转录病毒载体

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摘要

BackgroundRetroviral vectors are valuable tools for gene transfer. Particularly convenient are IRES-containing retroviral vectors expressing both the protein of interest and a marker protein from a single bicistronic mRNA. This coupled expression increases the relevance of tracking and/or selection of transduced cells based on the detection of a marker protein. pAP2 is a retroviral vector containing eGFP downstream of a modified IRES element of EMCV origin, and a CMV enhancer-promoter instead of the U3 region of the 5'LTR, which increases its efficiency in transient transfection. However, pAP2 contains a limited multicloning site (MCS) and shows weak eGFP expression, which previously led us to engineer an improved version, termed pPRIG, harboring: i) the wild-type ECMV IRES sequence, thereby restoring its full activity; ii) an optimized MCS flanked by T7 and SP6 sequences; and iii) a HA tag encoding sequence 5' of the MCS (pPRIG HAa/b/c).
机译:背景逆转录病毒载体是用于基因转移的有价值的工具。特别方便的是含有IRES的逆转录病毒载体,它可以从单个双顺反子mRNA表达目的蛋白和标记蛋白。基于标记蛋白的检测,这种偶联表达增加了追踪和/或选择转导细胞的相关性。 pAP2是一种逆转录病毒载体,在EMCV起源的修饰IRES元件下游包含eGFP,并含有CMV增强子启动子而不是5'LTR的U3区域,从而提高了其在瞬时转染中的效率。然而,pAP2包含有限的多克隆位点(MCS),并显示弱的eGFP表达,这以前使我们设计出了改良的版本,称为pPRIG,其中包含:i)野生型ECMV IRES序列,从而恢复了其完整活性; ii)优化的MCS,两侧为T7和SP6序列; iii)MCS的HA标签编码序列5'(pPRIG HAa / b / c)。

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