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Correlation between transgen expression and plasmid DNA loss in mouse liver

机译:小鼠肝脏中转基因表达与质粒DNA丢失的相关性

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Background Transgene expression from plasmid DNA is dependent on the expression efficiency per plasmid and the amount of intranuclear plasmid. In the present study, intranuclear dispositions of two types of plasmid DNAs (i.e. the pCpGfree and pLIVE plasmids) that maintain transgene expression in mouse liver were analyzed. In addition, the relationship between transgene expression and plasmid stability in the nucleus was examined. Methods First, the pCpGfree and pLIVE plasmid DNAs, bearing the mouse secreted alkaline phosphatase (Seap) gene, were administered into mouse liver by the hydrodynamics-based method. Next, various Seap-plasmid DNAs containing different promoters, upstream and downstream sequences, and backbones were injected into mice, and both SEAP expression and plasmid DNA amounts were monitored for 28 days. Results At the 14- and 28-day time points, the amount of the pCpGfree plasmid DNA was one order of magnitude less than that of the pLIVE plasmid. Meanwhile, the expression efficiency per plasmid was one order of magnitude more efficient for the pCpGfree plasmid DNA. Moreover, the administration of various Seap-plasmid DNAs revealed that negative correlations exist between plasmid stability and SEAP expression level. Conclusions The results obtained suggest that the pCpGfree plasmid is unstable from the viewpoint of quantity and maintains transgene expression by its high expression efficiency and also that transgene expression negatively affects the stability of plasmid DNA.
机译:背景来自质粒DNA的转基因表达取决于每个质粒的表达效率和核内质粒的量。在本研究中,分析了在小鼠肝脏中维持转基因表达的两种类型的质粒DNA(即pCpGfree和pLIVE质粒)的核内分布。另外,检查了转基因表达与核中质粒稳定性之间的关系。方法首先,通过基于流体动力学的方法,将带有小鼠分泌的碱性磷酸酶(Seap)基因的pCpGfree和pLIVE质粒DNA注入小鼠肝脏。接下来,将含有不同启动子,上游和下游序列以及骨架的各种Seap质粒DNA注入小鼠,并监测SEAP表达和质粒DNA量28天。结果在第14天和第28天的时间点,无pCpGG的质粒DNA的量比pLIVE质粒少了一个数量级。同时,每个质粒的表达效率对于不含pCpGG的质粒DNA的效率要高一个数量级。此外,各种Seap质粒DNA的管理表明质粒稳定性和SEAP表达水平之间存在负相关。结论所得结果表明,从数量上看,pCpGfree质粒是不稳定的,并且由于其高表达效率而保持转基因表达,并且转基因表达对质粒DNA的稳定性有负面影响。

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