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Plasmid DNA Mono-Ion Complex for in Vivo Sustainable Gene Expression

机译:用于体内可持续基因表达的质粒DNA单离子复合物

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To cleave biocompatible poly(ethylene glycol) (PEG) from the mono-ion complex (MIC) for sustainable cellular uptake in vivo, ω-amide-pentylimidazolium end-modified PEG with an ester bond, that is, APe-Im-E-PEG, has been synthesized. The hydrolysis of the resulting APe-Im-E-PEG proceeded during the incubation for 2 weeks under physiological conditions, which was confirmed by gel filtration chromatography. APe-Im-E-PEG formed the MIC with plasmid DNA (pDNA), assessed by agarose gel retardation assay. Furthermore, dynamic light scattering measurement and transmission electron microscopy observations have estimated that the particle size of the resulting MIC was approximately 30 nm, with a rather flexible structure. The APe-Im-E-PEG/pDNA MIC incubated for 2 weeks exhibited hemolytic activity at endosomal pH, presumably because the pH-sensitive carboxyl groups revealed after the hydrolysis of an ester bond of APe-Im-E-PEG. The APe-Im-E-PEG/pDNA MIC enhanced the gene expression 2 weeks after transfection in vivo by intramuscular administration in mice. Consequently, in vivo sustainable gene expression has been achieved by the molecular design of APe-Im-E-PEG for cellular uptake and endosomal escape proceeded by temporal hydrolysis of the ester bond.
机译:为了从单离子复合物(MIC)中裂解出生物相容性的聚乙二醇(PEG),以实现可持续的体内细胞摄取,ω-酰胺-戊咪唑鎓末端修饰的带有酯键的PEG,即APe-Im-E- PEG,已经合成。在生理条件下温育2周期间,所得APe-Im-E-PEG的水解进行,这通过凝胶过滤色谱法确认。 APe-Im-E-PEG与质粒DNA(pDNA)形成了MIC,通过琼脂糖凝胶阻滞分析评估。此外,动态光散射测量和透射电子显微镜观察估计,所得MIC的粒径约为30nm,具有相当柔性的结构。孵育2周的APe-Im-E-PEG / pDNA MIC在内体pH值下表现出溶血活性,大概是因为在APe-Im-E-PEG的酯键水解后出现了对pH敏感的羧基。 APe-Im-E-PEG / pDNA MIC通过在小鼠体内肌肉内转染2周后增强了基因表达。因此,已经通过APe-Im-E-PEG的分子设计实现了体内可持续的基因表达,该分子设计用于通过酯键的暂时水解进行的细胞摄取和内体逸出。

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