Platform of Biopharmacy, Faculty of Pharmacy, Université de Montréal, H3T 1J4, Canada.
Platform of Biopharmacy, Faculty of Pharmacy, Université de Montréal, H3T 1J4, Canada; Research Center and Pharmacy Department, Hôpital du Sacré-Coeur de Montréal, H4J 1C5, Canada.
J Pharm Biomed Anal. 2020 Oct 25;190:113521. doi: 10.1016/j.jpba.2020.113521. Epub 2020 Aug 15.
A sensitive and selective high-performance liquid chromatographic method coupled to tandem mass spectrometry was developed and validated for the quantification of morphine, hydromorphone, fentanyl, midazolam and propofol and their metabolites morphine-3-β-d-glucuronide, morphine-6-β-d-glucuronide, hydromorphone-3-β-d-glucuronide, 1'-hydroxymidazolam-β-d-glucuronide, α-hydroxymidazolam and 4-hydroxymidazolam in human plasma using potassium oxalate/sodium fluoride mixture as anticoagulant. Human plasma samples (0.4 mL) to which were added a mixture of eleven deuterated internal standards were subjected to solid phase extraction using a mixed-mode polymeric Oasis PRiME MCX in 96-well format. Propofol was selectively eluted and further derivatized using 2-Fluoro-1-methylpyridinium p-toluenesulfonate, whereas the remaining 10 analytes were eluted separately and further concentrated. The derivatized propofol was analyzed separately in a second injection. The analytes were chromatographically separated on a Kinetex phenyl-hexyl analytical column in gradient elution mode, using a mobile phase consisting of aqueous ammonium formate/formic acid buffer and methanol. The overall run time was 8 min. Detection was performed using an AB/SCIEX 4000 QTRAP instrument with positive electrospray ionization employing scheduled multiple reaction monitoring mode. The lower limits of quantification ranged from 0.02 to 5 ng/mL depending on the analyte. Calibration curves covered a concentration range of 1000× in all cases but 1'-hydroxymidazolam-β-d-glucuronide where it covered a range of 500 × . The validated method was accurate and precise, the intra-day accuracy and precision of quality control samples (4 concentration levels, n = 6 each) being within 91.5-112 % and 1.3-13.2 % (coefficient of variation), respectively, and inter-day (n = 24; 4 days) accuracy and precision of quality control samples (3 concentration levels) being within 94.8-103.5 % and 3.2-11.2 % (coefficient of variation). Mean absolute extraction recoveries were above 60 % for all compounds, except for hydromorphone-3-β-d-glucuronide (44 %) and for 1'-hydroxymidazolam-β-d-glucuronide (33 %). Internal standard corrected matrix effect ranged from -4.8 to 3.8 % in normal plasma and in plasma containing 1 % hemolyzed blood. Analytes were stable (above 90 %) in plasma and blood for 19 h at 22 °C, in blood for 90 h at 5 °C, in plasma for 60 days at -20 °C, for 4 months at -70 °C and after three freeze-thaw cycles, and in the injection solvent for at least 3 days in the autosampler. The present method is successfully being applied in a multicenter clinical study for the analysis of plasma samples from patients in intensive care units from a number of Canadian hospitals.
建立并验证了一种灵敏、选择性的高效液相色谱-串联质谱法,用于定量检测人血浆中的吗啡、氢吗啡酮、芬太尼、咪达唑仑和丙泊酚及其代谢物吗啡-3-β-d-葡萄糖醛酸、吗啡-6-β-d-葡萄糖醛酸、氢吗啡酮-3-β-d-葡萄糖醛酸、1'-羟基咪达唑仑-β-d-葡萄糖醛酸、α-羟基咪达唑仑和 4-羟基咪达唑仑,采用草酸钾/氟化钠混合物作为抗凝剂。将添加了 11 种氘代内标混合物的人血浆样品(0.4 mL)进行固相萃取,采用 96 孔格式混合模式聚合物 Oasis PRiME MCX。选择性洗脱丙泊酚,并用 2-氟-1-甲基吡啶对甲苯磺酸盐进一步衍生化,而其余 10 种分析物则分别洗脱并进一步浓缩。衍生化的丙泊酚在第二次进样中单独分析。分析物在 Kinetex 苯基-己基分析柱上以梯度洗脱模式进行色谱分离,流动相由含有氨甲酸铵/甲酸缓冲液和甲醇的水溶液组成。整个运行时间为 8 分钟。采用 AB/SCIEX 4000 QTRAP 仪器进行检测,采用正电喷雾电离,采用预定多重反应监测模式。根据分析物的不同,定量下限范围为 0.02-5 ng/mL。校准曲线的浓度范围均为 1000×,但 1'-羟基咪达唑仑-β-d-葡萄糖醛酸的浓度范围为 500×。验证后的方法准确、精密,质控样品(4 个浓度水平,n=6)的日内精密度和准确度分别在 91.5-112%和 1.3-13.2%(变异系数)之间,日间(n=24;4 天)准确度和精密度分别在 94.8-103.5%和 3.2-11.2%(变异系数)之间。除氢吗啡酮-3-β-d-葡萄糖醛酸(44%)和 1'-羟基咪达唑仑-β-d-葡萄糖醛酸(33%)外,所有化合物的绝对提取回收率均高于 60%。内标校正的基质效应在正常血浆和含 1%溶血血的血浆中为-4.8%至 3.8%。分析物在 22°C 下血浆中稳定(超过 90%)19 小时,在 5°C 下血液中稳定 90 小时,在-20°C 下血浆中稳定 60 天,在-70°C 下稳定 4 个月,在 3 次冻融循环后,在自动进样器中的进样溶剂中至少稳定 3 天。该方法已成功应用于加拿大多家医院重症监护病房患者血浆样本的多中心临床研究。
