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使用超高效液相色谱-高分辨率质谱法检测马毛中的合成代谢类固醇和雄激素类固醇及其酯类。

Detection of anabolic and androgenic steroids and/or their esters in horse hair using ultra-high performance liquid chromatography-high resolution mass spectrometry.

作者信息

Kwok Karen Y, Choi Timmy L S, Kwok Wai Him, Wong Jenny K Y, Wan Terence S M

机构信息

Racing Laboratory, The Hong Kong Jockey Club, Sha Tin Racecourse, Sha Tin, N.T., Hong Kong, China.

Racing Laboratory, The Hong Kong Jockey Club, Sha Tin Racecourse, Sha Tin, N.T., Hong Kong, China.

出版信息

J Chromatogr A. 2017 Apr 14;1493:76-86. doi: 10.1016/j.chroma.2017.03.007. Epub 2017 Mar 6.

Abstract

Anabolic and androgenic steroids (AASs) are a class of prohibited substances banned in horseracing at all times. The common approach for controlling the misuse of AASs in equine sports is by detecting the presence of AASs and/or their metabolites in urine and blood samples using gas chromatography-mass spectrometry (GC-MS) and liquid chromatography-mass spectrometry (LC-MS). This approach, however, often falls short as the duration of effect for many AASs are longer than their detection time in both urine and blood. As a result, there is a high risk that such AASs could escape detection in their official race-day samples although they may have been used during the long period of training. Hair analysis, on the other hand, can afford significantly longer detection windows. In addition, the identification of synthetic ester derivatives of AASs in hair, particularly for the endogenous ones, can provide unequivocal proof of their exogenous origin. This paper describes the development of a sensitive method (at sub to low parts-per-billion or ppb levels) for detecting 48 AASs and/or their esters in horse hair using ultra-high performance liquid chromatography-high resolution mass spectrometry (UHPLC-HRMS). Decontaminated horse hair was pulverised and subjected to in-situ liquid-liquid extraction in a mixture of hexane - ethyl acetate (7:3, v/v) and phosphate buffer (0.1M, pH 9.5), followed by additional clean-up using mixed-mode solid-phase extraction. The final extract was analysed using UHPLC-HRMS in the positive electrospray ionisation (ESI) mode with both full scan and parallel reaction monitoring (PRM). This method was validated for qualitative identification purposes. Validation data, including method specificity, method sensitivity, extraction recovery, method precision and matrix effect are presented. Method applicability was demonstrated by the successful detection and confirmation of testosterone propionate in a referee hair sample. To our knowledge, this was the first report of a comprehensive screening method for detecting as many as 48 AASs and/or their esters in horse hair. Moreover, retrospective analysis of non-targeted AASs and/or their esters was made feasible by re-examining the full scan UHPLC-HRMS data acquired.

摘要

合成代谢类固醇和雄激素类固醇(AASs)是赛马运动中一直被禁止的一类物质。控制马类运动中AASs滥用的常用方法是使用气相色谱 - 质谱联用仪(GC-MS)和液相色谱 - 质谱联用仪(LC-MS)检测尿液和血液样本中AASs及其代谢物的存在。然而,这种方法常常存在不足,因为许多AASs的作用持续时间比它们在尿液和血液中的检测时间长。因此,尽管这些AASs可能在长时间的训练期间被使用,但它们在官方比赛日样本中仍有很高的逃脱检测的风险。另一方面,毛发分析可以提供显著更长的检测窗口。此外,在毛发中鉴定AASs的合成酯衍生物,特别是内源性的,可以明确证明它们的外源性来源。本文描述了一种使用超高效液相色谱 - 高分辨率质谱联用仪(UHPLC-HRMS)检测马毛中48种AASs及其酯类的灵敏方法(检测限低至十亿分之几或ppb水平)。将经过去污处理的马毛粉碎,在己烷 - 乙酸乙酯(7:3,v/v)和磷酸盐缓冲液(0.1M,pH 9.5)的混合物中进行原位液 - 液萃取,然后使用混合模式固相萃取进行进一步净化。最终提取物在正电喷雾电离(ESI)模式下,采用全扫描和平行反应监测(PRM),通过UHPLC-HRMS进行分析。该方法已针对定性鉴定目的进行了验证。文中给出了包括方法特异性、方法灵敏度、萃取回收率、方法精密度和基质效应在内的验证数据。通过在一份裁判毛发样本中成功检测和确证丙酸睾酮,证明了该方法的适用性。据我们所知,这是首篇关于检测马毛中多达48种AASs及其酯类的综合筛查方法的报告。此外,通过重新检查所采集的全扫描UHPLC-HRMS数据,对非靶向AASs及其酯类进行回顾性分析成为可能。

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