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Optimization of DNA delivery by three classes of hybrid nanoparticle/DNA complexes

机译:通过三类杂化纳米颗粒/ DNA复合物优化DNA传递

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摘要

Plasmid DNA encoding a luciferase reporter gene was complexed with each of six different hybrid nanoparticles (NPs) synthesized from mixtures of poly (D, L-lactide-co-glycolide acid) (PLGA 50:50) and the cationic lipids DOTAP (1, 2-Dioleoyl-3-Trimethyammonium-Propane) or DC-Chol {3β-[N-(N', N'-Dimethylaminoethane)-carbamyl] Cholesterol}. Particles were 100-400 nm in diameter and the resulting complexes had DNA adsorbed on the surface (>out), encapsulated (>in), or DNA adsorbed and encapsulated (>both). A luciferase reporter assay was used to quantify DNA expression in 293 cells for the uptake of six different NP/DNA complexes. Optimal DNA delivery occurred for 105 cells over a range of 500 ng - 10 μg of NPs containing 20-30 μg DNA per 1 mg of NPs. Uptake of DNA from NP/DNA complexes was found to be 500-600 times as efficient as unbound DNA. Regression analysis was performed and lines were drawn for DNA uptake over a four week interval. NP/DNA complexes with adsorbed NPs (>out) showed a large initial uptake followed by a steep slope of DNA decline and large angle of declination; lines from uptake of adsorbed and encapsulated NPs (>both) also exhibited a large initial uptake but was followed by a gradual slope of DNA decline and small angle of declination, indicating longer times of luciferase expression in 293 cells. NPs with encapsulated DNA only (>in), gave an intermediate activity. The latter two effects were best seen with DOTAP-NPs while the former was best seen with DC-Chol-NPs. These results provide optimal conditions for using different hybrid NP/DNA complexes in vitro and in the future, will be tested in vivo.
机译:将编码萤光素酶报告基因的质粒DNA与由聚D,L-丙交酯-乙交酯乙交酯酸(PLGA 50:50)和阳离子脂质DOTAP(1, 2-二油酰基-3-三甲基铵-丙烷)或DC-Chol {3β-[N-(N',N'-二甲基氨基乙烷)-氨基甲酰基]胆固醇}。颗粒的直径为100-400 nm,所得复合物的表面(> out )吸附有DNA,包裹(> in )包裹了DNA,(>两者)。萤光素酶报告基因分析用于量化293细胞中DNA的表达,以摄取六种不同的NP / DNA复合物。在500 ng-10μgNP的范围内,对于10 5 细胞而言,最佳的DNA递送发生在每1 mg NP中包含20-30μgDNA。发现从NP / DNA复合物中摄取DNA的效率是未结合DNA的500-600倍。进行回归分析,并画出四周间隔的DNA摄取线。 NP / DNA与被吸附的NPs(> out )的复合物显示出较大的初始吸收,随后DNA下降的斜率大且偏角大。吸附和包裹的NPs(>两者)的摄取也显示出较大的初始摄取,但随后的DNA下降斜率逐渐减小,偏角较小,这表明荧光素酶在293细胞中的表达时间更长。仅具有封装的DNA(> in )的NP具有中等活性。使用DOTAP-NP最好看到后两种效果,而使用DC-Chol-NP最好看到前两种效果。这些结果为在体外使用不同的杂化NP / DNA复合物提供了最佳条件,将来将在体内进行测试。

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