Solid nano-in-nanoparticles for potential delivery of siRNA

细胞毒性 化学 纳米颗粒 生物物理学 小干扰RNA 基因沉默 乙二醇 纳米技术 材料科学 体外 生物化学 转染 生物 基因 有机化学
作者
Orit Amsalem,Taher Nassar,Sandrine Benhamron,Philip Lazarovici,Simon Benita,Eylon Yavin
出处
期刊:Journal of Controlled Release [Elsevier BV]
卷期号:257: 144-155 被引量:34
标识
DOI:10.1016/j.jconrel.2016.05.043
摘要

siRNA-based therapeutics possess great potential to treat a wide variety of genetic disorders. However, they suffer from low cellular uptake and short half-lives in blood circulation; issues that remain to be addressed. This work is, to the best of our knowledge, the first to report the production of solid nano-in-nanoparticles, termed double nano carriers (DNCs) by means of the innovative technology of nano spray drying. DNCs (with a median size of 580–770 nm) were produced by spraying at low temperatures (50 °C) to prevent damage to heat-sensitive biomacromolecules like siRNA. DNCs consisting of Poly (d,l-lactide-co-glycolide) used as a wall material, encapsulating 20% human serum albumin primary nanoparticles (PNPs) loaded with siRNA, were obtained as a dry nanoparticulate powder with smooth spherical surfaces and a unique inner morphology. Incubation of pegylated or non-pegylated DNCs under sink conditions at 37 °C, elicited a controlled release profile of the siRNA for up to 12 or 24 h, respectively, with a minimal burst effect. Prolonged incubation of pegylated DNCs loaded with active siRNA (anti EGFR) in an A549 epithelial cell culture monolayer did not induce any apparent cytotoxicity. A slow degradation of the internalized DNCs by the cells was also observed resulting in the progressive release of the siRNA for up to 6 days, as corroborated by laser confocal microscopy. The structural integrity and silencing activity of the double encapsulated siRNA were fully preserved, as demonstrated by HPLC, gel electrophoresis, and potent RNAi activity of siRNA extracted from DNCs. These results demonstrate the potential use of DNCs as a nano drug delivery system for systemic administration and controlled release of siRNA and potentially other sensitive bioactive macromolecules.
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