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基于气相色谱串联质谱法对合成代谢类固醇勃拉睾酮的推测质谱裂解途径进行代谢鉴定。

Metabolic Identification Based on Proposed Mass Fragmentation Pathways of the Anabolic Steroid Bolasterone by Gas Chromatography Tandem Mass Spectrometry.

作者信息

Muresan Anca Raluca, Rahaman Khandoker Asiqur, Rafique Farzana Binte, Son Junghyun, Kang Min-Jung, Kwon Oh-Seung

机构信息

Division of Bio-Medical Science & Technology, KIST School, University of Science and Technology, Seoul, South Korea.

Center for Advanced Biomolecular Recognition, Korea Institute of Science and Technology, Seoul, South Korea.

出版信息

Drug Test Anal. 2025 May 19. doi: 10.1002/dta.3903.

DOI:10.1002/dta.3903
PMID:40386947
Abstract

Bolasterone (7α,17α-dimethyl-androsta-4-en-17β-ol-3-one) was registered on the World Anti-Doping Agency's Prohibited list of substances. This study was aimed at evaluating the metabolism of bolasterone through in vitro (liver microsomes) and in vivo (rat urine) experiments to propose mass fragmentation pathways of the metabolites by gas chromatography-quadrupole tandem mass spectrometry (GC-EI-MS/MS). Their plausible chemical structures were suggested based on their fragmentation pathways to overcome the lack of available authentic standards. A total of 12 metabolites (5 mono-hydroxylated M1 to M5 and 7 di-hydroxylated M6 to M12) after trimethylsilylation were observed. Key diagnostic ions included m/z 403 (mono-hydroxylated) and m/z 491 (di-hydroxylated) with m/z 143, indicating an intact D ring (M1 to M5, M7, M9, M10, M11). Hydroxylation at the D ring (M6, M12) was characterized by ions m/z 231 or 219. Hydroxylation at the A (M5, M7) or B (M2/M3, M10) rings corresponded to m/z 281 and hydroxylation at C12 of the C ring (M4, M10) was indicated by m/z 285. Based on the comparison with bolasterone analogues such as testosterone and methyltestosterone and the interpretation of fragmentation pathways, the mono-hydroxylation metabolites M1 (at C11), M2/M3 (at C6), M4 (at C12), M5 (at C2), and di-hydroxylation metabolites M6 (at C11 and C16), M7 (at C2 and C11), M10 (at C6 and C12), and M12 (at C12 and C16) were proposed. The hydroxylation sites of M8, M9, and M11 could not be determined. This data can be useful for identifying hydroxylated metabolites by interpreting mass spectra of anabolic steroids with no standards available.

摘要

勃拉睾酮(7α,17α - 二甲基 - 雄甾 - 4 - 烯 - 17β - 醇 - 3 - 酮)被列入世界反兴奋剂机构的禁用物质清单。本研究旨在通过体外(肝微粒体)和体内(大鼠尿液)实验评估勃拉睾酮的代谢情况,利用气相色谱 - 四极杆串联质谱法(GC - EI - MS/MS)提出代谢产物的质量碎裂途径。基于其碎裂途径推测出它们可能的化学结构,以弥补缺乏可用标准品的不足。经三甲基硅烷化后,共观察到12种代谢产物(5种单羟基化的M1至M5和7种双羟基化的M6至M12)。关键诊断离子包括m/z 403(单羟基化)和m/z 491(双羟基化)以及m/z 143,表明D环完整(M1至M5、M7、M9、M10、M11)。D环羟基化(M6、M12)的特征离子为m/z 231或m/z 219。A环(M5、M7)或B环(M2/M3、M10)的羟基化对应m/z 281,C环C12位的羟基化(M4、M10)由m/z 285表示。通过与睾酮和甲基睾酮等勃拉睾酮类似物进行比较并结合碎裂途径的解释,提出了单羟基化代谢产物M1(C11位)、M2/M3(C6位)、M4(C12位)、M5(C2位)以及双羟基化代谢产物M6(C11和C16位)、M7(C2和C11位)、M10(C6和C12位)和M12(C12和C16位)。M8、M9和M11的羟基化位点无法确定。这些数据对于在没有标准品可用的情况下通过解释合成代谢类固醇的质谱来鉴定羟基化代谢产物可能会有所帮助。

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