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A novel in vitro delivery system for assessing the biological integrity of protein upon release from PLGA microspheres.

机译:一种新颖的体外递送系统,用于评估从PLGA微球释放后蛋白质的生物学完整性。

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PURPOSE: The development of a novel in vitro system is required to assess the stability and release kinetics of a protein microsphere formulation used for drug delivery to the brain. METHODS: Microspheres containing lysozyme as model protein were prepared using a (w/o/w) emulsion-solvent evaporation process. Both the active and total (active + inactive) encapsulation efficiencies and release profiles were determined. The biologic activity of lysozyme was measured using bacterial cell lysis; total protein content was measured using a 125I-radiolabel. A novel in vitro apparatus was developed to determine kinetics over a sustained time period (>30 days). RESULTS: The microencapsulation technique allowed an entrapment of active lysozyme at 80 +/- 4% and a sustained (>42 days) in vitro release. The kinetics study showed that the novel in vitro system was able to detect the release of low amounts (ng) of protein. To improve the stability of the protein within microspheres and allow the release of biologically active lysozyme, a basic additive ( Mg(OH)2 ) was successfully encapsulated. CONCLUSIONS: This novel in vitro system was appropriate to study protein microsphere release kinetics. In addition, the model is cost-effective and mimes brain physiological conditions more closely than previous models.
机译:目的:需要开发一种新型的体外系统来评估用于药物递送至大脑的蛋白质微球制剂的稳定性和释放动力学。方法:采用(w / o / w)乳液-溶剂蒸发法制备了以溶菌酶为模型蛋白的微球。确定了活性和总(活性+非活性)包封效率和释放曲线。用细菌细胞裂解法测定溶菌酶的生物活性。总蛋白含量使用125 I-放射性标记进行测量。开发了一种新颖的体外仪器来确定持续时间(> 30天)内的动力学。结果:微囊化技术可以捕获80 +/- 4%的活性溶菌酶,并可以持续(> 42天)体外释放。动力学研究表明,新型体外系统能够检测出少量(ng)蛋白质的释放。为了提高蛋白质在微球体内的稳定性并释放生物活性溶菌酶,已成功地封装了一种碱性添加剂(Mg(OH)2)。结论:这种新颖的体外系统适用于研究蛋白质微球的释放动力学。此外,该模型具有成本效益,并且比以前的模型更能模仿大脑的生理状况。

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