Development and validation of a high-performance liquid chromatography method with fluorescence detection for the quantification of the resistance protein P-gp in cancer cells

IF 2.5 3区 医学 Q2 BIOCHEMICAL RESEARCH METHODS Journal of Chromatography B Pub Date : 2025-03-01 Epub Date: 2025-01-21 DOI:10.1016/j.jchromb.2025.124475
Elodie Gay, Maxime Dubois, Manon Roux, Antoine Goisnard, Marie Depresle, Mahchid Bamdad, Pierre Daumar, Emmanuelle Mounetou
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Abstract

A method using high-performance liquid chromatography coupled with fluorescence detection (HPLC-FLD) was developed and validated to quantify the innovative tool LightSpot®-FL-1, a selective permeability-glycoprotein (P-gp)-targeted fluorescent conjugate used to measure P-gp expression in cell samples. Quantifying P-gp is a major challenge in oncology as its overexpression in many cancer cells results in Multidrug Resistance (MDR) associated with chemotherapy failure. To develop the method reported herein, both sample preparation and analysis parameters were investigated. Optimal chromatographic conditions were achieved with 5 µL injections at a 1 mL/min flow rate on a reversed-phase Zorbax® Eclipse Plus 3.5 µm C18 column (150 × 4.6 mm) with isocratic acetonitrile/water (85/15, by volume) elution. Detection was performed with 505 nm excitation and 510 nm emission wavelengths. Validation studies were designed and performed according to the International Council for Harmonization (ICH) guidelines for bioanalytical method validation. The limit of quantification (LOQ) and limit of detection (LOD) were determined to be 0.5 and 0.2 nmol/L, respectively. The linearity range was demonstrated between 10 and 500 nmol/L, and the trueness and precision of the method were validated. Good stability was shown in three relevant analytical conditions. The greenness of the developed method was also demonstrated with the AGREE, AGREEprep and MoGAPI tools. Finally, the rapid, precise and sensitive validated analytical method was successfully applied to determine the difference in P-gp expression in three cancer cell lines: DU4475, CCRF-CEM and KG-1a.
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建立高效液相色谱法和荧光检测法定量测定癌细胞中耐药蛋白P-gp。
采用高效液相色谱-荧光检测(HPLC-FLD)的方法开发并验证了创新工具LightSpot®-FL-1的定量方法。LightSpot®-FL-1是一种选择性渗透糖蛋白(P-gp)靶向荧光偶联物,用于测量细胞样品中P-gp的表达。由于P-gp在许多癌细胞中的过度表达导致与化疗失败相关的多药耐药(MDR),因此定量P-gp是肿瘤学的主要挑战。为了建立本文报道的方法,对样品制备和分析参数进行了研究。在Zorbax®Eclipse Plus 3.5µm C18反相柱(150 × 4.6 mm)上,以1 mL/min流速,5µL进样,等容乙腈/水(85/15,体积)洗脱,获得最佳色谱条件。检测波长为505 nm,发射波长为510 nm。验证研究是根据国际统一理事会(ICH)生物分析方法验证指南设计和实施的。定量限和检出限分别为0.5 nmol/L和0.2 nmol/L。在10 ~ 500 nmol/L的线性范围内,验证了方法的正确性和精密度。在三个相关分析条件下均表现出良好的稳定性。通过AGREE、AGREEprep和MoGAPI工具验证了所开发方法的环保性。最后,成功应用快速、精确、灵敏的分析方法测定了DU4475、CCRF-CEM和KG-1a三种癌细胞株中P-gp的表达差异。
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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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