Institute for Pharmacy and Food Chemistry, University of Würzburg, Am Hubland, 97074 Würzburg, Germany.
University of Würzburg Medical Center, Department of Internal Medicine II, Oberdürrbacher Str. 6, 97080 Würzburg, Germany.
J Pharm Biomed Anal. 2022 Mar 20;211:114623. doi: 10.1016/j.jpba.2022.114623. Epub 2022 Jan 29.
Personalized dosing of kinase inhibitors (KI) might be beneficial in oral anti-cancer therapy to overcome individual pharmacokinetic variability. Volumetric absorptive microsampling (VAMS) has emerged as an attractive alternative compared to conventional invasive sampling methods enabling remote and frequent specimen collection. Therefore, an LC-MS/MS VAMS method was developed and validated to monitor drug exposure of ten KI from 20 µL dried capillary blood. The assay includes the KI cabozantinib, dabrafenib, nilotinib, and osimertinib with a calibration range of 6-1500 ng/mL and afatinib, axitinib, bosutinib, lenvatinib, ruxolitinib and trametinib within a range of 2-500 ng/mL. Using acetonitrile containing isotope labelled internal standards (IS) as solid-liquid extraction solvent, analytes and IS were detected by multiple reaction monitoring (MRM) after electro-spray ionization (ESI) in positive ionization mode after chromatographic separation using a phenyl-hexyl column. The method was validated according to the FDA and EMA guidelines for bioanalytical method validation and in accordance with the guideline of the International Association for Therapeutic Drug Monitoring and Clinical Toxicology for dried blood spot-based methods. The calibration model was linear and reproducible for all KI (R> 0.994). Furthermore, the validation demonstrated that the VAMS method is accurate, precise, and sensitive. The method fulfilled the acceptance criteria for matrix effects, recovery, carry over, selectivity as well as for the haematocrit effect and all substances proved to be stable in dried condition for at least six weeks at room temperature. In vitro experiments using spiked venous blood were conducted to establish a VAMS-to-plasma conversion factor for each analyte for comparison of VAMS and plasma concentrations. The method was successfully used in a real-life setting demonstrating its applicability in clinical routine. VAMS concentrations of afatinib, cabozantinib, dabrafenib, nilotinib, ruxolitinib and trametinib were assessed in capillary blood samples collected from either trained healthcare professionals or patients at home.
个体化给药的激酶抑制剂(KI)可能有益于口服抗癌治疗,以克服个体药代动力学的变异性。与传统的侵入性采样方法相比,体积吸收微采样(VAMS)已成为一种有吸引力的替代方法,能够进行远程和频繁的样本采集。因此,开发并验证了一种 LC-MS/MS VAMS 方法,用于监测 20µL 干毛细血管血中 10 种 KI 的药物暴露情况。该方法包括 KI 卡博替尼、达拉非尼、尼洛替尼和奥希替尼,校准范围为 6-1500ng/mL,阿法替尼、阿昔替尼、博舒替尼、仑伐替尼、鲁索替尼和曲美替尼的校准范围为 2-500ng/mL。采用乙腈作为固相萃取溶剂,其中含有同位素标记的内标(IS)。分析物和 IS 在电喷雾电离(ESI)后,经正离子模式检测,经苯基-己基色谱柱分离后,采用多反应监测(MRM)检测。该方法按照 FDA 和 EMA 生物分析方法验证指南以及国际治疗药物监测和临床毒理学协会(IATDMCT)关于干血斑方法的指南进行验证。校准模型对所有 KI 均呈线性和重现性(R>0.994)。此外,验证结果表明,VAMS 方法准确、精密且灵敏。该方法满足基质效应、回收率、交叉污染、选择性以及红细胞压积效应的接受标准,所有物质在室温下干态下至少稳定 6 周。使用加标静脉血进行的体外实验,建立了每个分析物的 VAMS 与血浆浓度的转换因子,用于比较 VAMS 和血浆浓度。该方法已成功应用于实际环境,证明了其在临床常规中的适用性。从经过培训的医护人员或在家中的患者采集毛细血管血样,评估阿法替尼、卡博替尼、达拉非尼、尼洛替尼、鲁索替尼和曲美替尼的 VAMS 浓度。
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