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首个用于定量检测人血液、唾液和尿液中 9R-和 9S-六氢大麻酚及其代谢物的 LC-MS/MS 立体选择性生物分析方法。

The first LC-MS/MS stereoselective bioanalytical methods to quantitatively detect 9R- and 9S-hexahydrocannabinols and their metabolites in human blood, oral fluid and urine.

机构信息

Department of Excellence-Biomedical Sciences and Public Health, Università Politecnica delle Marche, 60121 Ancona, Italy.

National Centre on Addiction and Doping, Istituto Superiore di Sanità, 00161 Rome, Italy.

出版信息

J Pharm Biomed Anal. 2024 Mar 15;240:115918. doi: 10.1016/j.jpba.2023.115918. Epub 2023 Dec 13.

DOI:10.1016/j.jpba.2023.115918
PMID:38181553
Abstract

A sensitive LC-MS/MS method for the simultaneous quantification of the (9 R)- and (9 S)- hexahydrocannabinols (HHCs), and their metabolites, in human urine, oral fluid (OF) and blood samples were developed, validated and used to the biological samples of volunteers. The analytes were extracted from 100 μL human samples. An isocratic elution mode with methanol was used for chromatographic separation of (9 R)- and (9 S)-HHC on an immobilized amylose tris(3-chloro-5-methylphenylcarbamate)-based chiral column Lux i-Amylose-3. The flow-rate of the mobile phase was 0.5 mL/min. An isocratic elution mode of methanol and water (80/20, v/v) was used for chromatographic separation of metabolites of (9 R)- and (9 S)-HHC on a Lux AMP chiral column (with a proprietary chiral selector) at a flow rate of 0.5 mL/min. MS/MS analysis was performed in positive ionization mode for HHC epimers, while in negative ionization mode was used for metabolites of HHCs. The calibration curves for HHCs and their metabolites in human samples ranged from 0.25- 240 ng mL and 1 - 100 ng mL, respectively, with determination coefficients (r) of ≥ 0.99. All analytes were stable at room temperature, 4 °C, in the autosampler (+10 °C) and -20 °C for 24 h, after three freeze/thaw cycles, and when stored at -20 °C up to one week after quality control (QC) sample preparation (concentration differences less than 20% with respect to time zero response), in blood, urine and OF.

摘要

建立并验证了一种灵敏的 LC-MS/MS 方法,用于同时定量分析人尿、唾液和血液样本中(9R)-和(9S)-六氢大麻酚(HHC)及其代谢物。分析物从 100μL 人样本中提取。在固定化直链淀粉三(3-氯-5-甲基苯基氨基甲酸酯)基手性柱 Lux i-Amylose-3 上,甲醇等度洗脱模式用于(9R)-和(9S)-HHC 的色谱分离。流动相流速为 0.5mL/min。甲醇和水(80/20,v/v)等度洗脱模式用于 Lux AMP 手性柱(具有专有的手性选择剂)上(9R)-和(9S)-HHC 代谢物的色谱分离,流速为 0.5mL/min。HHC 差向异构体采用正离子化模式进行 MS/MS 分析,而 HHC 代谢物采用负离子化模式进行分析。HHC 和其代谢物在人样品中的校准曲线范围分别为 0.25-240ng/mL 和 1-100ng/mL,决定系数(r)均≥0.99。所有分析物在室温下、4°C、自动进样器(+10°C)和-20°C 下 24h 内、经过三个冻融循环以及在-20°C 下储存长达 QC 样品制备后一周内稳定(相对于零时响应的浓度差异小于 20%),在血液、尿液和唾液中均稳定。

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