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Formulation development of lyophilized, long-term stable siRNA/oligoaminoamide polyplexes

机译:制剂冻干,长期稳定siRNA /寡氨基酰胺多用途的开发

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摘要

Polyplexes based on precise oligoaminoamides exhibited promising results in non-viral siRNA delivery. However, one serious limitation is insufficient stability of polyplexes in liquid, which raises the demand for lyophilized, long-term stable formulations. Two different siRNA/oligoaminoamide polyplexes were prepared. Freeze-thaw experiments were performed, in order to test various formulations containing sucrose, trehalose, lactosucrose, and hydroxypropyl-β-cyclodextrin for their cryoprotective potential and to investigate the influence of the oligoaminoamide structure on particle stability. Selected formulations were lyophilized and tested for storage stability up to 6 months. Moreover, reconstitution of the lyophilisates in reduced volume as a technique to prepare higher concentration formulations was studied. Samples were analyzed for particle size, gene silencing, cytotoxicity, turbidity, subvisible particles, osmolarity, residual moisture content, glass transition temperature, and morphology. Depending on the oligoaminoamide, siRNA polyplexes maintained particle size and gene silencing efficiency in the absence or presence of low amounts (7%) of stabilizers after freeze-thawing, lyophilization, and reconstitution. Particle stability was highly dependent on the oligoaminoamide used, but independent of the presence of cysteines that form intra-particular disulfide bridges. In contrast to all other excipients, hydroxypropyl-β-cyclodextrin did not provide sufficient stability. For lyophilized 5%/10% sucrose and 7% lactosucrose formulations, long-term stability was demonstrated at 40 °C with retained particle size, retained gene silencing activity, unchanged turbidity values, low numbers of subvisible particles, low residual moisture level, and sufficiently high glass transition temperature. Hence, this work is a promising approach in order to provide long-term stable siRNA polyplex formulations that are ready to use after a simple reconstitution step.
机译:基于精确的寡聚基亚酰胺的多重表现出有希望的非病毒siRNA递送的结果。然而,一种严重的限制是液体中的多用途稳定性,这提高了对冻干的需求,长期稳定的制剂。制备两种不同的siRNA /寡氨基酰胺酰胺。进行冻融实验,以测试含有蔗糖,海藻糖,乳糖蔗糖和羟丙基-β-环糊精的各种制剂,用于它们的冷冻保护潜力,并研究寡氨基酰胺结构对颗粒稳定性的影响。将选定的制剂冻干并测试储存稳定性长达6个月。此外,研究了作为制备更高浓度制剂的技术减少体积的冻干物的重构。分析样品进行粒度,基因沉默,细胞毒性,浊度,劣质颗粒,渗透压,残留含量,玻璃化转变温度和形态学。取决于寡聚氨基酰胺,在冷冻解冻,冻干和重构后,SiRNA多用途在没有或存在的低量(7%)稳定剂的情况下保持粒度和基因沉默效率。颗粒稳定性高度依赖于所用的寡核苷酸,但是与形成特定的二硫桥的半胱氨酸的存在无关。与所有其他赋形剂相比,羟丙基-β-环糊精没有提供足够的稳定性。对于冻干的5%/ 10%蔗糖和7%乳孢子制剂,长期稳定性在40℃下,保留的粒度,保留基因沉默活性,不变的浊度值,低数量的劣质颗粒,低残留的水分水平,以及足够高的玻璃化转变温度。因此,这项工作是一种有希望的方法,以便提供在简单的重构步骤之后准备使用的长期稳定的siRNA多络合物制剂。

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