开发和验证超高效液相色谱串联质谱方法，用于定量分析人血浆和各种小鼠生物样品中的抗寄生虫药物 DNDI-6148。

IF 2.8 3区医学 Q2 BIOCHEMICAL RESEARCH METHODS

Journal of Chromatography B Pub Date : 2024-11-12 DOI:10.1016/j.jchromb.2024.124377

Wietse M. Schouten , Katrien Van Bocxlaer , Hilde Rosing , Alwin D.R. Huitema , Jos H. Beijnen , Jadel M. Kratz , Charles E. Mowbray , Thomas P.C. Dorlo

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引用次数: 0

摘要

DNDI-6148是一种治疗皮肤利什曼病（CL）的新型口服药物，这种寄生虫病被忽视，影响着全世界的贫困人口。有必要进行临床前靶点药代动力学（PK）研究，以评估皮肤利什曼病寄生虫实际接触 DNDI-6148 的情况。为了促进这些研究，我们开发并验证了一种反相超高效液相色谱-串联质谱（UPLC-MS/MS）方法，用于定量检测相关目标部位 PK 样品中的 DNDI-6148 药物，该方法符合国际人用药品技术要求协调理事会（ICH）关于生物分析方法验证的 M10 指南。对替代生物指标人 K2EDTA 血浆、酶消化缓冲液和皮肤微量透析液进行了全面验证。对小鼠 K2EDTA 血浆和组织进行了部分验证。使用基于胶原酶 A 的酶解均质化工作流程对包括小鼠皮肤、肝脏和脾脏在内的组织样本进行了均质化。与常用的机械匀浆法相比，该方法从皮肤中提取 DNDI-6148 的效果提高了 2.9 倍。随后对所有生物基质进行了蛋白质沉淀。每种方法都使用了一种替代生物基质，其范围是根据其预期应用专门制定的，结果是人体 K2EDTA 血浆、酶消化缓冲液和微量透析液的线性浓度范围分别为 5.00-2000 纳克/毫升、2.00-1000 纳克/毫升和 3.00-600 纳克/毫升。在所有浓度水平上，每种生物基质在运行内和运行间的准确度和精密度均在 15% 以内。基质效应不影响 DNDI-6148 的测定，因为 DNDI-6148 的稳定同位素标记内标有效地补偿了这些基质效应。所有方法的总回收率在 73.5 % 到 81.3 % 之间（CV ≤4.5%）。在各种条件下，DNDI-6148 在所有测试的生物样品中都很稳定。不过，在均质化过程中，DNDI-6148 的浓度有所下降，而内标物对其进行了适当的校正。在一项使用CL感染小鼠模型进行的临床前靶点PK研究中，证明了该方法适用于未来涉及DNDI-6148的临床前研究。

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Development and validation of ultra-performance liquid chromatography tandem mass spectrometry methods for the quantitative analysis of the antiparasitic drug DNDI-6148 in human plasma and various mouse biomatrices

DNDI-6148 is a promising new oral drug for the treatment of cutaneous leishmaniasis (CL), a parasitic neglected tropical disease that affects impoverished populations worldwide. Preclinical target site pharmacokinetics (PK) studies are necessary to evaluate the actual exposure to DNDI-6148 of Leishmania parasites in the skin. To facilitate these investigations, we have developed and validated a reversed phase ultra-performance liquid chromatography coupled to tandem mass spectrometry (UPLC-MS/MS) method to quantify DNDI-6148 in relevant target site PK samples, adhering to the relevant International Council for Harmonisation of Technical Requirements for Pharmaceuticals for Human Use (ICH) M10 guideline on bioanalytical method validation. Full validation was performed for the surrogate biomatrices human K₂EDTA plasma, enzymatic digestion buffer and skin microdialysate. Partial validation was conducted for mouse K₂EDTA plasma and tissues. The tissue samples, including mouse skin, liver and spleen, were homogenized using a collagenase A-based enzymatic homogenization workflow. This method was found to be 2.9-fold more effective in extracting DNDI-6148 from skin than the commonly used mechanical homogenization. Protein precipitation was subsequently carried out for all biomatrices. A surrogate biomatrix was used for each method and the range was specifically developed for its intended application, resulting in a linear concentration range of 5.00–2000 ng/mL, 2.00–1000 ng/mL, and 3.00–600 ng/mL for human K₂EDTA plasma, enzymatic digestion buffer and microdialysate, respectively. Each biomatrix had intra- and inter-run accuracy and precision within 15 % for all concentration levels. Matrix effects did not affect the determination of DNDI-6148, since the stable isotopically-labelled internal standard for DNDI-6148 effectively compensated for these matrix effects. Total recovery across all methods was between 73.5 % and 81.3 % (CV ≤4.5 %). DNDI-6148 was stable under various conditions in all the tested biomatrices. However, a decrease in its concentration was observed during homogenization, for which the internal standard corrected adequately. The suitability of the method for use in future preclinical research involving DNDI-6148 was demonstrated in a preclinical target site PK study using a CL-infected murine model.

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来源期刊

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.