A liquid chromatography-tandem mass spectrometry analysis of nine cytochrome P450 probe drugs and their corresponding metabolites in human serum and urine
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  • 作者:Elena Puris ; Markku Pasanen ; Mikko Gynther…
  • 关键词:LC ; MS/MS ; Cocktail approach ; CYP ; Pharmacokinetics ; In vivo ; Sample preparation
  • 刊名:Analytical and Bioanalytical Chemistry
  • 出版年:2017
  • 出版时间:January 2017
  • 年:2017
  • 卷:409
  • 期:1
  • 页码:251-268
  • 全文大小:
  • 刊物类别:Chemistry and Materials Science
  • 刊物主题:Analytical Chemistry; Biochemistry, general; Laboratory Medicine; Characterization and Evaluation of Materials; Food Science; Monitoring/Environmental Analysis;
  • 出版者:Springer Berlin Heidelberg
  • ISSN:1618-2650
  • 卷排序:409
文摘
Cocktail phenotyping using specific probe drugs for cytochrome P450 (CYP) enzymes provides information on the real-time activity of multiple CYPs. We investigated different sample preparation techniques and validated a liquid chromatography-tandem mass spectrometry (LC-MS/MS) method with simple protein precipitation for the analysis of nine CYP probe drugs and their metabolites in human serum and urine. Specific CYP probe drugs (melatonin, CYP1A2; nicotine, CYP2A6; bupropion, CYP2B6; repaglinide, CYP2C8; losartan, CYP2C9; omeprazole, CYP2C19 and CYP3A4; dextromethorphan, CYP2D6; chlorzoxazone, CYP2E; midazolam, CYP3A4) and their main metabolites, with the exception of 3′-hydroxyrepaglinide, were quantified in human serum and urine using the developed LC-MS/MS method. The analytical method was fully validated showing high selectivity, linearity, acceptable accuracy (85–115 %) and precision (2–19 %) and applied to a pharmacokinetic study in four healthy volunteers after oral administration of drugs given as a cocktail. All probe drugs and their metabolites (totally 19 analytes) were detected and quantified from human serum and urine over the time range of 1 to 6 h after oral administration. Therefore, the proposed method is applicable for drug interaction and CYP phenotyping studies utilizing a cocktail approach.

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