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用于反兴奋剂目的的血清中内源性类固醇及其II相代谢物同时定量的单运行超高效液相色谱-串联质谱法。

Single-run UHPLC-MS/MS method for simultaneous quantification of endogenous steroids and their phase II metabolites in serum for anti-doping purposes.

作者信息

Ponzetto Federico, Parasiliti-Caprino Mirko, Gesmundo Iacopo, Marinelli Lorenzo, Nonnato Antonello, Nicoli Raul, Kuuranne Tiia, Mengozzi Giulio, Ghigo Ezio, Settanni Fabio

机构信息

Division of Endocrinology, Diabetes and Metabolism, Department of Medical Sciences, University of Turin; Turin, Italy.

Division of Endocrinology, Diabetes and Metabolism, Department of Medical Sciences, University of Turin; Turin, Italy.

出版信息

Talanta. 2023 Apr 1;255:124218. doi: 10.1016/j.talanta.2022.124218. Epub 2022 Dec 28.

Abstract

Anti-doping rule violations related to the abuse of endogenous anabolic androgenic steroids can be currently discovered by the urinary steroidal module of Athlete Biological Passport. Since this powerful tool is still subjected to some limitations due to various confounding factors altering the steroid profile, alternative strategies have been constantly proposed. Among these, the measurement of blood concentrations of endogenous steroid hormones by LC-MS is currently of increasing interest in anti-doping, bringing significant advantages for the detection of testosterone abuse in females and in individuals with deletion of UGT2B17 enzyme. Although various research groups have made significant efforts in method development, there is currently no accepted or harmonized anti-doping method for quantitative analysis of the various testosterone doping markers in blood. In this study we present a UHPLC-MS/MS method for the quantification of major circulating steroid hormones together with an extended panel of glucuro- and sulpho-conjugated phase II metabolites of androgens. Chromatographic setup was optimized by comparing the performance of three different C18 stationary phases and by the careful selection of mobile phases with the aim of separating all the target steroids, including numerous isomeric/isobaric compounds. MS parameters were fine-tuned to obtain the sensitivity needed for measuring the target analytes, that show specific serum concentrations ranging from low pg/mL for less abundant compounds to μg/mL for sulpho-conjugated steroids. Finally, sample preparation protocol was developed for the extraction of steroid hormones from 200 μL of serum and the performance was evaluated in terms of extraction recovery and matrix effect. The final method was then applied to authentic serum samples collected from healthy volunteers (40 males and 40 females) at the Blood Bank of the City of Health and Science University Hospital of Turin. The analysis of these samples allowed to obtain results on serum concentrations of the targeted steroids, with particular emphasis on previously undiscovered phase II metabolites, such as the isomers of 5-androstane-3,17-diol glucuronide. This preliminary application also enabled measuring dihydrotestosterone sulphate in male samples, efficiently separating this analyte from its isomer, epiandrosterone sulphate, which circulates in blood at high concentrations. The promising results of this study are encouraging for the measurement of blood steroid profile markers in serum and plasma samples for Athlete Biological Passport purposes.

摘要

目前,运动员生物护照的尿液甾体模块能够发现与滥用内源性合成代谢雄激素类固醇相关的反兴奋剂规则违规行为。由于各种混杂因素会改变类固醇谱,这个强大的工具仍然存在一些局限性,因此人们不断提出替代策略。其中,通过液相色谱 - 质谱法测量内源性类固醇激素的血药浓度在反兴奋剂领域目前越来越受到关注,这为检测女性和UGT2B17酶缺失个体中的睾酮滥用带来了显著优势。尽管各个研究团队在方法开发方面付出了巨大努力,但目前尚无用于定量分析血液中各种睾酮兴奋剂标志物的公认或统一的反兴奋剂方法。在本研究中,我们提出了一种超高效液相色谱 - 串联质谱法,用于定量主要循环类固醇激素以及一组扩展的雄激素葡萄糖醛酸和硫酸酯结合的II相代谢物。通过比较三种不同C18固定相的性能并精心选择流动相,优化了色谱设置,目的是分离所有目标类固醇,包括众多同分异构体/同量异位化合物。对质谱参数进行了微调,以获得测量目标分析物所需的灵敏度,这些分析物的血清浓度范围从低丰度化合物的低皮克/毫升到硫酸酯结合类固醇的微克/毫升。最后,开发了从200微升血清中提取类固醇激素的样品制备方案,并从提取回收率和基质效应方面评估了其性能。然后将最终方法应用于从都灵市健康与科学大学医院血库收集的健康志愿者(40名男性和40名女性)的真实血清样本。对这些样本的分析得出了目标类固醇血清浓度的结果,特别关注了以前未发现的II相代谢物,如5 - 雄甾烷 - 3,17 - 二醇葡萄糖醛酸的异构体。这项初步应用还能够在男性样本中测量硫酸脱氢表雄酮,有效地将该分析物与其异构体硫酸表雄酮分离,硫酸表雄酮在血液中以高浓度循环。这项研究的令人鼓舞的结果对于为运动员生物护照目的测量血清和血浆样本中的血液类固醇谱标志物具有鼓舞作用。

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