4.4 Article

Detection of the designer benzodiazepine metizolam in urine and preliminary data on its metabolism

Journal

DRUG TESTING AND ANALYSIS
Volume 9, Issue 7, Pages 1026-1033

Publisher

WILEY
DOI: 10.1002/dta.2099

Keywords

benzodiazepines; metizolam; urine; metabolism; HLMs

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Designer benzodiazepines provide an attractive alternative to prescribed benzodiazepines for abuse purposes as they are readily available via the Internet without control. Metizolam was ordered via the Internet and a 2mg blue tablet was orally administered to a 54-year-old man. Urine samples were collected over 6days in polypropylene tubes. After liquid/liquid extraction at pH9.5, metizolam was analyzed by ultra-performance liquid chromatography-electrospray ionization-tandem mass spectrometry (UPLC-ESI-MS/MS) using a standard method devoted to benzodiazepines, and ions transitions, at m/z 328.9>275.0 and 328.9>300.0. Metizolam was detectable in hydrolyzed urine during the 46-h period, with concentrations always lower than 11ng/mL. About 0.3% of the initial dose was excreted in urines as total unchanged metizolam during the first 24h. The most relevant potential CYP- and UGT-dependent metabolites of metizolam were investigated in vitro using human liver microsome incubation and, subsequently, liquid chromatography coupled with quadrupole-time of flight mass spectrometry (UHPLC-Q-TOF-MS) analysis. Three mono-hydroxylated metabolites were produced including a hydroxylation compound at the 2-ethyl moiety of metizolam (M1) as quantitatively main metabolite, and a N-hydroxymetiazolam (M2). The structure of the third metabolite (M3) could not be elucidated because of a too low experimental production rate. Two authentic urine samples were analyzed using the same analytical method to search for metabolites of metizolam. M1, together with its glucuronide (M1-Glu), and M2 were observed in urine at the 8h mark, whereas only M1 and M1-Glu were still detected in urine at 30h post administration. Copyright (C) 2016 John Wiley & Sons, Ltd.

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