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载药微球用于化疗栓塞:药物释放的体外评价方法。

Sunitinib-eluting beads for chemoembolization: methods for in vitro evaluation of drug release.

机构信息

School of Pharmaceutical Sciences, University of Geneva, University of Lausanne, Quai Ernest Ansermet 30, 1211 Geneva 4, Switzerland.

Departments of Radiology and Interventional Radiology, CHUV Centre Hospitalier Universitaire Vaudois, Rue du Bugnon 46, 1011 Lausanne, Switzerland.

出版信息

Int J Pharm. 2015 Mar 30;482(1-2):68-74. doi: 10.1016/j.ijpharm.2014.11.041. Epub 2014 Nov 18.

DOI:10.1016/j.ijpharm.2014.11.041
PMID:25448554
Abstract

Drug-eluting microspheres are used for embolization of hypervascular tumors and allow for local controlled drug release. Although the drug release from the microspheres relies on fast ion-exchange, so far only slow-releasing in vitro dissolution methods have been correlated to in vivo data. Three in vitro release methods are assessed in this study for their potential to predict slow in vivo release of sunitinib from chemoembolization spheres to the plasma, and fast local in vivo release obtained in an earlier study in rabbits. Release in an orbital shaker was slow (t50%=4.5h, 84% release) compared to fast release in USP 4 flow-through implant cells (t50%=1h, 100% release). Sunitinib release in saline from microspheres enclosed in dialysis inserts was prolonged and incomplete (t50%=9 days, 68% release) due to low drug diffusion through the dialysis membrane. The slow-release profile fitted best to low sunitinib plasma AUC following injection of sunitinib-eluting spheres. Although limited by lack of standardization, release in the orbital shaker fitted best to local in vivo sunitinib concentrations. Drug release in USP flow-through implant cells was too fast to correlate with local concentrations, although this method is preferred to discriminate between different sphere types.

摘要

载药微球用于富血管肿瘤的栓塞,并允许局部控制药物释放。虽然微球中的药物释放依赖于快速的离子交换,但迄今为止,只有缓慢释放的体外溶解方法与体内数据相关联。本研究评估了三种体外释放方法,以评估它们预测舒尼替尼从化疗栓塞微球向血浆中缓慢体内释放的潜力,以及在之前的兔子体内研究中获得的快速局部体内释放。与 USP4 流动植入细胞中的快速释放(t50%=1h,100%释放)相比,在轨道摇床中的释放较慢(t50%=4.5h,84%释放)。由于药物通过透析膜扩散率低,包埋在透析膜中的微球中的舒尼替尼在盐水中的释放延长且不完全(t50%=9 天,68%释放)。低舒尼替尼血浆 AUC 与注射舒尼替尼载药微球后的释放情况最吻合。尽管由于缺乏标准化而受到限制,但轨道摇床中的释放最适合体内局部舒尼替尼浓度。USP 流动植入细胞中的药物释放速度太快,无法与体内局部浓度相关联,尽管这种方法更适合区分不同类型的微球。

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