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Erythropoietin-loaded solid lipid nanoparticles: Preparation, optimization, and in vivo evaluation

机译:促红细胞素加载的固体脂质纳米粒子:制备,优化和体内评价

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Solid lipid nanoparticle (SLN) is a promising approach for delivery of various drugs including proteins and peptides. However, the loading of hydrophilic drugs into the lipoid matrix of SLNs is challenging. The statistical design is a potential method facilitating the optimization of nanoparticles characteristics. In this study, the Box-Behnken design was conducted to optimize the preparation of Erythropoietin (EPO) loaded SLNs. Circular dichroism, size exclusion chromatography, SDS-PAGE, and ELISA tests were used to prove the compatibility of the process with the stability of EPO. In the controlled situation, EPO preserved its conformation and activity during the SLN preparation. Regarding the particle size, entrapment efficiency, and polydispersity index, an optimum formulation was obtained with 130 mg Span((R))80, 152.5 mu l EPO, and 1.9 min high-shear homogenization. Using the optimum condition, 280 nm sized SLNs with the narrow size distribution of 0.282 and entrapment efficiency of 43.4% were acquired. The in vitro cytotoxicity of optimum SLN formulation was conducted using MTT assay to show its safety on the evaluated cell line. The in vivo studies demonstrated that 2500 U EPO loaded SLN has similar or even better effects on elevating the RBC, hemoglobin, and hematocrit level compared to the 5000 U EPO solution. Generally, this study proposed a suitable EPO-loaded SLN preparation method as a potential drug delivery system for proteins.
机译:固体脂质纳米粒子(SLN)是一种有望的方法,用于递送包括蛋白质和肽在内的各种药物。然而,将亲水药物加入SLNS的脂质基质是具有挑战性的。统计设计是促进纳米颗粒特性优化的潜在方法。在这项研究中,进行了盒子的设计,以优化促红细胞生成素(EPO)的SLN的制备。圆形二色性,大小排除色谱,SDS-PAGE和ELISA测试用于证明该过程的兼容性与EPO的稳定性。在受控情况下,EPO在SLN准备期间保留了其构象和活动。关于粒度,夹带效率和多分散性指数,用130mg跨度((r))80,152.5μlPOO和1.9分钟高剪切均质化获得最佳制剂。采用最佳条件,收购了280nm尺寸的SLN,尺寸窄尺寸分布0.282,截留效率为43.4%。使用MTT测定法进行最佳SLN制剂的体外细胞毒性,以显示其对评估的细胞系的安全性。体内研究表明,与5000 u EPO溶液相比,2500 U opo载荷的SLN对升高RBC,血红蛋白和血细胞比容水平具有相似或甚至更好的影响。通常,该研究提出了一种合适的EPO加载的SLN制备方法作为蛋白质的潜在药物递送系统。

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