首页> 外文期刊>Journal of Controlled Release: Official Journal of the Controlled Release Society >Polycation-DNA complexes for gene delivery: a comparison of the biopharmaceutical properties of cationic polypeptides and cationic lipids
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Polycation-DNA complexes for gene delivery: a comparison of the biopharmaceutical properties of cationic polypeptides and cationic lipids

机译:用于基因传递的聚阳离子-DNA复合物:阳离子多肽和阳离子脂质的生物制药特性比较

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DNA plasmids formed particulate complexes with a variety of cationic polyamino acids and cationic lipids, which were used to transfect mammalian cells in culture. Complexation was studied by assaying for exclusion of ethidium using a fluorometric assay, which indicated that complexation with cationic polyamino acids took place with utilisation of the majority of charged functional groups. The particle sizes and zeta potentials of a range of complexes were determined. Generally polyamino acids formed uniform particles 80-120 nm in diameter in water, but their particle size increased on dilution of the particles in electrolytes or cell culture media. The efficiency of transfection was compared using complexes of pRSVlacZ, a reporter construct which expressed beta-galactosidase under the control of the Rous sarcoma virus promoter. Positively charged DNA/polyamino acid complexes were taken up by cells but required an endosomolytic agent, such as chloroquine, to facilitate transfection. Polyornithine complexes resulted in the highest levels of expression, in comparison with other homopolyamino acids (polyornithine>poly-L-lysine=poly-D-lysine>polyarginine). Copolyamino acids of lysine and alanine condensed DNA but were less active in transfection experiments. Copoly(L-Lys, L-Ala 1:1) was inactive even in the presence of chloroquine. In contrast DNA/cationic lipid complexes transfected cells spontaneously, and chloroquine did not improve the extent of expression, rather it usually reduced efficiency. There was little correlation between comparative efficiencies of lipid complexes between cell lines suggesting that the nature of the cell membrane and differences in mechanisms of internalisation were determinants of efficiency. In an effort to explore better cell culture models for gene delivery, monolayers of Caco-2 cells were transfected in filter culture. As the cells differentiated and formed a polarized monolayer, expression of beta-galactosidase was reduced until at day 27 expression was not significantly different from basal activity. The Caco-2 filter culture model merits further attention as a model of gene delivery to epithelial surfaces, such as would be encountered in the lung after inhalation. (C) 1998 Elsevier Science B.V. [References: 30]
机译:DNA质粒与各种阳离子聚氨基酸和阳离子脂质形成颗粒复合物,可用于转染培养物中的哺乳动物细胞。通过使用荧光测定法测定乙锭的排阻作用来研究络合,这表明与阳离子聚氨基酸的络合是利用大多数带电官能团进行的。测定了一系列配合物的粒度和ζ电势。通常,聚氨基酸在水中形成直径为80-120 nm的均匀颗粒,但是随着颗粒在电解质或细胞培养基中的稀释,它们的粒径会增加。使用pRSVlacZ的复合物比较了转染的效率,pRSVlacZ是一种在Rous肉瘤病毒启动子的控制下表达β-半乳糖苷酶的报告基因构建体。带正电荷的DNA /聚氨基酸复合物被细胞吸收,但需要内溶菌剂(例如氯喹)以促进转染。与其他均聚氨基酸相比,聚鸟氨酸复合物导致最高的表达水平(聚鸟氨酸>聚-L-赖氨酸=聚-D-赖氨酸>聚精氨酸)。赖氨酸和丙氨酸的共聚氨基酸浓缩DNA,但在转染实验中活性较低。即使在存在氯喹的情况下,共聚(L-Lys,L-Ala 1:1)也没有活性。相反,DNA /阳离子脂质复合物可自发转染细胞,而氯喹并不能提高表达程度,而通常会降低效率。细胞系之间脂质复合物的比较效率之间几乎没有相关性,表明细胞膜的性质和内化机制的差异是效率的决定因素。为了探索用于基因递送的更好的细胞培养模型,在滤膜培养中转染了单层Caco-2细胞。随着细胞分化并形成极化的单层,β-半乳糖苷酶的表达降低,直到第27天表达与基础活性无明显差异。 Caco-2过滤器培养模型作为基因传递到上皮表面的模型值得进一步关注,例如吸入后在肺中会遇到的情况。 (C)1998 Elsevier Science B.V. [参考:30]

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