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Adjusting the attB Site in Donor Plasmid Improves the Efficiency of Phi C31 Integrase System

机译:调节供体质粒中的attB位点可提高Phi C31整合酶系统的效率

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摘要

Phi C31 integrase, a site-specific recombinase, can catalyze integration of circular DNA bearing attB site into pseudo attP sites in mammalian genomes. However, the integration efficiency mediated by integrase is relatively low. Our study centered on the investigation of the impact of the position, orientation, and number of attBs in the donor plasmid on the efficiency of Phi C31 integrase system. Donor plasmids bearing various types of attBs (including forward and reverse directions, tandem, and intersperse) and reporter enhanced green fluorescent protein (EGFP) were constructed. The plasmids plus helper plasmid encoding integrase were co-transfected into HeLa cells. After G418 selection, the resistant cell colonies were counted for calculating chromosomal integration frequency. EGFP expression was detected by fluorescence-activated cell sorter and enzyme-linked immuno-sorbent assay analysis. The results showed that efficiency of integration mediated by integrase accounted for 70% +/- 7.1% of total integration events in the transfected HeLa cells. Compared with a forward orientation of attB in donor plasmid, a reverse direction of attB or interspersed attBs showed 1.5- or 2.8-fold increase in integration efficiency, respectively, while tandem attBs in donor plasmids caused a decreased efficiency of integration. We conclude that the adjustment of attB sites in donor plasmids may be of value for gene therapy and routine genetic engineering by using Phi C31 integrase system.
机译:Phi C31整合酶是一种位点特异性重组酶,可催化将带有attB位点的环状DNA整合到哺乳动物基因组中的伪attP位点。然而,由整合酶介导的整合效率相对较低。我们的研究集中于调查供体质粒中attB的位置,方向和数目对Phi C31整合酶系统效率的影响。构建了带有各种attB(包括正向和反向,串联和穿插)和报道基因增强的绿色荧光蛋白(EGFP)的供体质粒。将质粒和编码整合酶的辅助质粒共转染到HeLa细胞中。选择G418后,计数抗性细胞集落以计算染色体整合频率。通过荧光激活细胞分选仪和酶联免疫吸附测定分析检测EGFP表达。结果表明,整合酶介导的整合效率在转染的HeLa细胞中占总整合事件的70%+/- 7.1%。与供体质粒中attB的正向相比,attB或散布的attB的反向分别显示整合效率提高1.5或2.8倍,而供体质粒中的串联attB导致整合效率降低。我们得出的结论是,通过使用Phi C31整合酶系统,对供体质粒中attB位点的调节对于基因治疗和常规基因工程可能具有价值。

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