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人尿中安非他酮及其氧化、还原和葡糖醛酸代谢物的综合立体选择性液相色谱/质谱联用测定法的开发、验证及应用

Development, validation and application of a comprehensive stereoselective LC/MS-MS assay for bupropion and oxidative, reductive, and glucuronide metabolites in human urine.

作者信息

Teitelbaum Aaron M, Flaker Alicia M, Kharasch Evan D

机构信息

Department of Anesthesiology, Washington University in St. Louis, St. Louis, MO 63110, United States.

Department of Anesthesiology, Washington University in St. Louis, St. Louis, MO 63110, United States; Department of Biochemistry and Molecular Biology, Washington University in St. Louis, St. Louis, MO 63110, United States; The Center for Clinical Pharmacology, St. Louis College of Pharmacy and Washington University School of Medicine St. Louis, MO 63110, United States.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2016 Aug 1;1027:239-53. doi: 10.1016/j.jchromb.2016.05.036. Epub 2016 May 24.

Abstract

A stereoselective assay was developed for the quantification of bupropion and oxidative, reductive, and glucuronide metabolites (16 analytes total) in human urine. Initially, authentic glucuronide standards obtained from commercial sources were found to be incorrectly labeled with regard to stereochemistry; the correct stereochemistry was unequivocally reassigned. A trifurcated urine sample preparation and analysis procedure was employed for the stereoselective analysis of bupropion, hydroxybupropion, erythrohydrobupropion, and threohydrobupropion enantiomers, and hydroxybupropion, erythrohydrobupropion and threohydrobupropion β-d-glucuronide diastereomers in urine. Method 1 stereoselectively analyzed bupropion (R and S), and unconjugated free hydroxybupropion (R,R and S,S), erythrohydrobupropion (1R,2S and 1S,2R), and threohydrobupropion (1R,2R and 1S,2S) using chiral chromatography with an α1-acid glycoprotein column. Because no hydroxybupropion β-d-glucuronide standards were commercially available, method 2 stereoselectively analyzed total hydroxybupropion aglycones (R,R and S,S-hydroxybupropion) after urine hydrolysis by β-glucuronidase. Hydroxybupropion β-d-glucuronide (R,R and S,S) urine concentrations were calculated as the difference between total and free hydroxybupropion (R,R and S,S) concentrations. Due to incomplete β-glucuronidase hydrolysis of erythrohydrobupropion and threohydrobupropion β-d-glucuronide diastereomers, method 3 stereoselectively analyzed intact erythrohydrobupropion and threohydrobupropion β-d-glucuronide diastereomers using C18 column chromatography. All analytes were quantified by positive ion electrospray tandem mass spectrometry. The assay was fully validated over analyte-specific concentrations. Intra- and inter assay precision were within 15% for each analyte. The limits of quantification for bupropion (R and S), hydroxybupropion (R,R and S,S), threohydrobupropion (1S,2S and 1R,2R), erythrohydrobupropion (1R,2S and 1S,2R) were 10, 50, 100, and 100ng/mL, respectively. The limits of quantification for (1R,2R)-threohydrobupropion β-d-glucuronide, (1S,2S)-threohydrobupropion β-d-glucuronide, and (1R,2R)-erythrohydrobupropion β-d-glucuronide were each 50ng/mL. Due to the abundance of bupropion and metabolites in human urine, no efforts were made to optimize sensitivity. All analytes were stable following freeze thaw cycles at -80°C. This assay was applicable to clinical pharmacokinetic investigations of bupropion in patients and to in vitro metabolism of the primary bupropion metabolites to their glucuronides.

摘要

开发了一种立体选择性测定法,用于定量人尿中安非他酮及其氧化、还原和葡糖醛酸代谢物(共16种分析物)。最初,发现从商业来源获得的葡糖醛酸标准品在立体化学方面标记错误;明确重新指定了正确的立体化学结构。采用了一种三叉式尿液样品制备和分析程序,用于对安非他酮、羟基安非他酮、赤藓醇羟基安非他酮和苏阿糖醇羟基安非他酮对映体,以及尿液中的羟基安非他酮、赤藓醇羟基安非他酮和苏阿糖醇羟基安非他酮β - d - 葡糖醛酸非对映体进行立体选择性分析。方法1使用α1 - 酸性糖蛋白柱的手性色谱法立体选择性分析安非他酮(R和S)、未结合的游离羟基安非他酮(R,R和S,S)、赤藓醇羟基安非他酮(1R,2S和1S,2R)和苏阿糖醇羟基安非他酮(1R,2R和1S,2S)。由于没有商业可得的羟基安非他酮β - d - 葡糖醛酸标准品,方法2在尿液经β - 葡糖醛酸酶水解后立体选择性分析总羟基安非他酮苷元(R,R和S,S - 羟基安非他酮)。羟基安非他酮β - d - 葡糖醛酸(R,R和S,S)的尿液浓度通过总羟基安非他酮(R,R和S,S)浓度与游离羟基安非他酮(R,R和S,S)浓度之差计算得出。由于赤藓醇羟基安非他酮和苏阿糖醇羟基安非他酮β - d - 葡糖醛酸非对映体的β - 葡糖醛酸酶水解不完全,方法3使用C18柱色谱法立体选择性分析完整的赤藓醇羟基安非他酮和苏阿糖醇羟基安非他酮β - d - 葡糖醛酸非对映体。所有分析物通过正离子电喷雾串联质谱法定量。该测定法在特定分析物浓度范围内得到了充分验证。每种分析物的批内和批间精密度均在15%以内。安非他酮(R和S)、羟基安非他酮(R,R和S,S)、苏阿糖醇羟基安非他酮(1S,2S和1R,2R)、赤藓醇羟基安非他酮(1R,2S和1S,2R)的定量限分别为10、50、100和100 ng/mL。(1R,2R) - 苏阿糖醇羟基安非他酮β - d - 葡糖醛酸、(1S,2S) - 苏阿糖醇羟基安非他酮β - d - 葡糖醛酸和(1R,2R) - 赤藓醇羟基安非他酮β - d - 葡糖醛酸的定量限均为50 ng/mL。由于人尿中安非他酮和代谢物含量丰富,未进行灵敏度优化。所有分析物在 - 80°C冻融循环后均稳定。该测定法适用于安非他酮在患者中的临床药代动力学研究,以及主要安非他酮代谢物向其葡糖醛酸的体外代谢研究。

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