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通过免疫亲和纯化和液相色谱-高分辨质谱/质谱对人血浆中生长激素释放激素进行定性鉴定。

Qualitative identification of growth hormone-releasing hormones in human plasma by means of immunoaffinity purification and LC-HRMS/MS.

作者信息

Knoop Andre, Thomas Andreas, Fichant Eric, Delahaut Philippe, Schänzer Wilhelm, Thevis Mario

机构信息

Institute for Biochemistry-Center for Preventive Doping Research, German Sport University Cologne, Am Sportpark Müngersdorf 6, 50933, Cologne, Germany.

Laboratoire d'Hormonologie, C.E.R. Groupe-Département Santé, Rue du Point du jour 8, 6900, Marloie, Belgium.

出版信息

Anal Bioanal Chem. 2016 May;408(12):3145-53. doi: 10.1007/s00216-016-9377-3. Epub 2016 Feb 15.

DOI:10.1007/s00216-016-9377-3
PMID:26879649
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4830873/
Abstract

The use of growth hormone-releasing hormones (GHRHs) is prohibited in sports according to the regulations of the World Anti-Doping Agency (WADA). The aim of the present study was to develop a method for the simultaneous detection of four different GHRHs and respective metabolites from human plasma by means of immunoaffinity purification and subsequent nano-ultrahigh performance liquid chromatography-high resolution/high accuracy (tandem) mass spectrometry. The target analytes included Geref (Sermorelin), CJC-1293, CJC-1295, and Egrifta (Tesamorelin) as well as two metabolites of Geref and CJC-1293, which were captured from plasma samples using a polyclonal GHRH antibody in concert with protein A/G monolithic MSIA™ D.A.R.T.'S® (Disposable Automation Research Tips) prior to separation and detection. The method was fully validated and found to be fit for purpose considering the parameters specificity, linearity, recovery (19-37%), lower limit of detection (<50 pg/mL), imprecision (<20%), and ion suppression/enhancement effects. The analytes' stability and metabolism were elucidated using in vitro and in vivo approaches. EDTA blood samples were collected from rats 2, 4, and 8 h after intravenous administration of GHRH (one compound per test animal). All intact substances were detected for at least 4 h but no anticipated metabolite was confirmed in laboratory rodents' samples; conversely, a Geref metabolite (GHRH3-29) was found in a human plasma sample collected after subcutaneous injection of the drug to a healthy male volunteer. The obtained results demonstrate that GHRHs are successfully detected in plasma using an immunoaffinity-mass spectrometry-based method, which can be applied to sports drug testing samples. Further studies are however required and warranted to account for potential species-related differences in metabolism and elimination of the target analytes.

摘要

根据世界反兴奋剂机构(WADA)的规定,生长激素释放激素(GHRHs)在体育运动中被禁止使用。本研究的目的是开发一种方法,通过免疫亲和纯化以及随后的纳米超高效液相色谱-高分辨率/高精度(串联)质谱法,同时检测人血浆中四种不同的GHRHs及其各自的代谢物。目标分析物包括Geref(舍莫瑞林)、CJC-1293、CJC-1295和Egrifta(替沙莫瑞林),以及Geref和CJC-1293的两种代谢物,在分离和检测之前,使用多克隆GHRH抗体与蛋白A/G整体式MSIA™ D.A.R.T.'S®(一次性自动化研究吸头)从血浆样本中捕获这些物质。该方法经过了全面验证,考虑到特异性、线性、回收率(19-37%)、检测下限(<50 pg/mL)、不精密度(<20%)和离子抑制/增强效应等参数,发现该方法符合要求。使用体外和体内方法阐明了分析物的稳定性和代谢情况。在给大鼠静脉注射GHRH(每只试验动物注射一种化合物)后2、4和8小时采集乙二胺四乙酸(EDTA)血样。所有完整物质至少检测到4小时,但在实验啮齿动物的样本中未确认有预期的代谢物;相反,在向一名健康男性志愿者皮下注射该药物后采集的人血浆样本中发现了一种Geref代谢物(GHRH3-29)。获得的结果表明,使用基于免疫亲和质谱的方法可成功在血浆中检测到GHRHs,该方法可应用于运动药物检测样本。然而,还需要并值得进行进一步研究,以考虑目标分析物在代谢和消除方面潜在的物种相关差异。

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