Development and validation of a UPLC-MS/MS method for rapid and simultaneous quantification of BPI-460372 and its metabolites BPI-460444 and BPI-460456 in human plasma

IF 2.8 3区 医学 Q2 BIOCHEMICAL RESEARCH METHODS
Jianwei Ren , Hongzhong Liu , Yufang Ma , Wei Tian , Qinqin Li , Zhen Wu , Mengzhao Wang , Xiaoyun Liu , Xin Zheng , Xiaohong Han
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Abstract

In cancer development and progression, the Hippo signaling pathway functions. The transcriptional enhanced associate domain (TEAD) stands out as a pivotal transcription factor within this pathway, and the suppression of TEAD represents a promising approach for cancer treatment. The primary aim of the study was to establish an analytical method for the concurrent quantification of a novel TEAD target inhibitor, BPI-460372, and its principal metabolites, BPI-460444 and BPI-460456, in human plasma. The chromatographic separation utilized a XSelect™ HSS C18 column (2.1 × 100 mm, 2.5 µm), while quantification was conducted on a SCIEX API 4000 mass spectrometer. 22 plasma samples were tested via the developed method. The calibration curve for BPI-460372 exhibited linearity from 2 to 2000 ng/mL, while its metabolites BPI-460444 and BPI-460456 had linearity between 1 and 1000 ng/mL (r > 0.99). The precision (RSD) was ≤ 17.1 %, and the accuracy (RE) fell within the range of −17.7 % to 15.0 %, all meeting acceptance criteria. The matrix effect was from 101.0 % to 105.8 %. The extraction recovery of analytes fell within the range of 96.8 % to 104.1 % with an RSD of less than 7.4 %. The developed method was effectively utilized in an advanced solid tumor patient, and the concentration trends of the three analytes in plasma were found to be largely consistent. The established analytical method showed great sensitivity, simplicity, accuracy, and reliability for the rapid and simultaneous analysis of the TEAD target inhibitor BPI-460372, alongside its major metabolites BPI-460444 and BPI-460456 in human plasma. This analytical method provided essential support for future clinical investigations and pharmacokinetic analysis.

Abstract Image

建立并验证一种UPLC-MS/MS方法,用于快速、同时定量检测人血浆中的BPI-460372及其代谢物BPI-460444和BPI-460456
在癌症的发生和发展过程中,Hippo 信号通路发挥着作用。转录增强关联结构域(TEAD)是该通路中的一个关键转录因子,抑制 TEAD 是一种很有前景的癌症治疗方法。本研究的主要目的是建立一种分析方法,用于同时定量检测人体血浆中的新型 TEAD 靶点抑制剂 BPI-460372 及其主要代谢物 BPI-460444 和 BPI-460456。色谱分离采用 XSelect™ HSS C18 色谱柱(2.1 × 100 mm,2.5 µm),定量采用 SCIEX API 4000 质谱仪。采用所开发的方法检测了 22 份血浆样品。BPI-460372的线性范围为2-2000 ng/mL,其代谢物BPI-460444和BPI-460456的线性范围为1-1000 ng/mL(r >0.99)。精密度(RSD)≤17.1%,准确度(RE)在-17.7%至15.0%之间,均符合接受标准。基质效应为 101.0 % 至 105.8 %。分析物的萃取回收率在 96.8 % 至 104.1 % 之间,RSD 小于 7.4 %。所建立的方法在晚期实体瘤患者中得到了有效的应用,血浆中三种分析物的浓度变化趋势基本一致。所建立的分析方法灵敏度高、简便、准确、可靠,可同时快速分析人血浆中的TEAD靶向抑制剂BPI-460372及其主要代谢物BPI-460444和BPI-460456。该分析方法为今后的临床研究和药代动力学分析提供了重要支持。
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来源期刊
Journal of Chromatography B
Journal of Chromatography B 医学-分析化学
CiteScore
5.60
自引率
3.30%
发文量
306
审稿时长
44 days
期刊介绍: The Journal of Chromatography B publishes papers on developments in separation science relevant to biology and biomedical research including both fundamental advances and applications. Analytical techniques which may be considered include the various facets of chromatography, electrophoresis and related methods, affinity and immunoaffinity-based methodologies, hyphenated and other multi-dimensional techniques, and microanalytical approaches. The journal also considers articles reporting developments in sample preparation, detection techniques including mass spectrometry, and data handling and analysis. Developments related to preparative separations for the isolation and purification of components of biological systems may be published, including chromatographic and electrophoretic methods, affinity separations, field flow fractionation and other preparative approaches. Applications to the analysis of biological systems and samples will be considered when the analytical science contains a significant element of novelty, e.g. a new approach to the separation of a compound, novel combination of analytical techniques, or significantly improved analytical performance.
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