开发 UPLC-MS/MS 方法，用于研究氟唑帕尼与姜黄素在大鼠体内的药代动力学相互作用

IF 3.1 3区医学 Q2 CHEMISTRY, ANALYTICAL

Journal of pharmaceutical and biomedical analysis Pub Date : 2024-07-28 DOI:10.1016/j.jpba.2024.116383

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引用次数: 0

摘要

Fuzuloparib是一种新型口服生物活性聚ADP核糖聚合酶抑制剂（PARPi），于2020年获中国药监局批准用于治疗对铂敏感的复发性卵巢癌、输卵管癌和原发性腹膜癌。本研究首次提出了一种快速、准确的超高效液相色谱-串联质谱（UPLC-MS/MS）方法，用于分析fuzuloparib及其主要代谢物（SHR165202）的含量，并在体外和体内研究fuzuloparib与姜黄素之间的药物相互作用。采用乙腈沉淀蛋白后，以乙腈和0.1%甲酸为流动相进行梯度洗脱，成功分离了fuzuloparib、SHR165202和talazoparib（内标物，IS）。结果表明，fuzuloparib和SHR165202分别在2-50 ng/mL和1-20 ng/mL的校准范围内线性关系良好。方法验证所需的精密度、准确度、稳定性、基质效应和提取回收率均符合《生物分析方法验证指南》的要求。在体外微粒体孵育实验中，姜黄素对大鼠肝脏微粒体（RLM）和人肝脏微粒体（HLM）中的福舒帕利均有抑制作用，其半最大抑制浓度（IC50）分别为10.54 μM和47.64 μM，相应的机制为非竞争性。此外，还通过分子对接验证了姜黄素对夫唑帕利的抑制机制。在大鼠药代动力学实验中，姜黄素显著改变了fuzuloparib的血浆暴露量，使fuzuloparib的AUC（0-t）和Cmax显著增加，CLz/F显著降低。此外，代谢物 SHR165202 的 AUC(0-t)、AUC(0-∞)、Tmax 和 Cmax 均显著增加，CLz/F 显著降低。这进一步支持了姜黄素可以抑制福舒帕尼代谢的观点。因此，在临床上联合使用氟唑帕尼和姜黄素时，建议监测氟唑帕尼的血浆水平，并密切关注不良反应。如有必要，应减少福舒帕尼的剂量。

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Development of UPLC–MS/MS method for studying the pharmacokinetic interactions of fuzuloparib with curcumin in rats

Fuzuloparib is a novel orally bioactive poly-ADP-ribose polymerase inhibitor (PARPi), which was approved by the Chinese Regulatory Agency (CRA) in 2020 for the treatment of platinum-sensitive recurrent ovarian, fallopian tube, and primary peritoneal cancers. This study firstly presents a rapid and accurate ultra performance liquid chromatography tandem mass spectrometry (UPLC-MS/MS) method for analyzing the levels of fuzuloparib and its major metabolite (SHR165202), and to investigate drug-drug interaction between fuzuloparib and curcumin in vitro and in vivo studies. After protein precipitation with acetonitrile, mobile phase consisted of acetonitrile and 0.1 % formic acid with a gradient elution was used to successfully separate fuzuloparib, SHR165202 and talazoparib (internal standard, IS). The results indicated that fuzuloparib and SHR165202 had good linearity over the calibration range of 2–50 ng/mL and 1–20 ng/mL, respectively. The precision, accuracy, stability, matrix effect, and extraction recovery required for methodological validation all complied with the requirements of the Bioanalytical Method Validation Guidelines. In vitro microsome incubation experiments, curcumin exhibited inhibitory effect on fuzuloparib in both rat liver microsomes (RLM) and human liver microsomes (HLM) with half-maximal inhibitory concentration (IC₅₀) value of 10.54 μM and 47.64 μM, respectively, and the corresponding mechanism was non-competitive. Furthermore, the inhibitory mechanism of curcumin on fuzuloparib was validated through molecular docking. In pharmacokinetic experiments in rats, curcumin significantly altered the plasma exposure of fuzuloparib, resulting in significant increases in AUC_(0-t) and C_max of fuzuloparib and a significant decrease in CL_z/F. Moreover, the metabolite SHR165202 showed significant increases in AUC_(0-t), AUC_(0-∞), T_max and C_max and a significant decrease in CL_z/F. This further supports the notion that curcumin could inhibit the metabolism of fuzuloparib. Therefore, when co-administering fuzuloparib and curcumin in clinic, it is recommended to monitor plasma levels of fuzuloparib and pay close attention to adverse effects. If necessary, the dose of fuzuloparib needs to be reduced.

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来源期刊

Journal of pharmaceutical and biomedical analysis 医学-分析化学

CiteScore

6.70

自引率

5.90%

发文量

588

审稿时长

37 days

期刊介绍： This journal is an international medium directed towards the needs of academic, clinical, government and industrial analysis by publishing original research reports and critical reviews on pharmaceutical and biomedical analysis. It covers the interdisciplinary aspects of analysis in the pharmaceutical, biomedical and clinical sciences, including developments in analytical methodology, instrumentation, computation and interpretation. Submissions on novel applications focusing on drug purity and stability studies, pharmacokinetics, therapeutic monitoring, metabolic profiling; drug-related aspects of analytical biochemistry and forensic toxicology; quality assurance in the pharmaceutical industry are also welcome. Studies from areas of well established and poorly selective methods, such as UV-VIS spectrophotometry (including derivative and multi-wavelength measurements), basic electroanalytical (potentiometric, polarographic and voltammetric) methods, fluorimetry, flow-injection analysis, etc. are accepted for publication in exceptional cases only, if a unique and substantial advantage over presently known systems is demonstrated. The same applies to the assay of simple drug formulations by any kind of methods and the determination of drugs in biological samples based merely on spiked samples. Drug purity/stability studies should contain information on the structure elucidation of the impurities/degradants.