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金属组学在药物开发中的应用:CE-ICP-MS 法在人血浆中对脂质体顺铂药物制剂的表征。

Metallomics in drug development: characterization of a liposomal cisplatin drug formulation in human plasma by CE-ICP-MS.

机构信息

Department of Pharmacy Faculty of Health and Medical Sciences, University of Copenhagen, Universitetsparken 2, 2100 Copenhagen, Denmark.

出版信息

Anal Bioanal Chem. 2013 Feb;405(6):1845-54. doi: 10.1007/s00216-012-6355-2. Epub 2012 Sep 30.

Abstract

A capillary electrophoresis inductively coupled plasma mass spectrometry method for separation of free cisplatin from liposome-encapsulated cisplatin and protein-bound cisplatin was developed. A liposomal formulation of cisplatin based on PEGylated liposomes was used as model drug formulation. The effect of human plasma matrix on the analysis of liposome-encapsulated cisplatin and intact cisplatin was studied. The presence of 1 % of dextran and 4 mM of sodium dodecyl sulfate in HEPES buffer was demonstrated to be effective in improving the separation of liposomes and cisplatin bound to proteins in plasma. A detection limit of 41 ng/mL of platinum and a precision of 2.1 % (for 10 μg/mL of cisplatin standard) were obtained. Simultaneous measurements of phosphorous and platinum allows the simultaneous monitoring of the liposomes, liposome-encapsulated cisplatin, free cisplatin and cisplatin bound to plasma constituents in plasma samples. It was demonstrated that this approach is suitable for studies of the stability of liposome formulations as leakage of active drug from the liposomes and subsequent binding to biomolecules in plasma can be monitored. This methodology has not been reported before and will improve characterization of liposomal drugs during drug development and in studies on kinetics.

摘要

建立了一种毛细管电泳电感耦合等离子体质谱法,用于分离游离顺铂、脂质体包裹的顺铂和蛋白结合的顺铂。以聚乙二醇化脂质体为模型药物制剂,研究了基于顺铂的脂质体制剂。研究了人血浆基质对脂质体包裹的顺铂和完整顺铂分析的影响。结果表明,在 HEPES 缓冲液中加入 1%的葡聚糖和 4mM 的十二烷基硫酸钠可有效改善血浆中脂质体与蛋白质结合的顺铂的分离效果。检测限为 41ng/ml 的铂,精密度为 2.1%(10μg/ml 的顺铂标准品)。磷和铂的同时测量允许同时监测血浆样品中的脂质体、脂质体包裹的顺铂、游离顺铂和与血浆成分结合的顺铂。结果表明,该方法适用于脂质体制剂稳定性的研究,因为可以监测活性药物从脂质体中泄漏并随后与血浆中的生物分子结合。这种方法以前没有报道过,将提高药物开发过程中以及动力学研究中对脂质体药物的表征。

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