首页> 外文期刊>Therapeutic Drug Monitoring >Screening procedure for detection of stimulant laxatives and/or their metabolites in human urine using gas chromatography-mass spectrometry after enzymatic cleavage of conjugates and extractive methylation.
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Screening procedure for detection of stimulant laxatives and/or their metabolites in human urine using gas chromatography-mass spectrometry after enzymatic cleavage of conjugates and extractive methylation.

机译:酶切裂解缀合物和萃取甲基化后,使用气相色谱-质谱法检测人尿中兴奋性泻药和/或其代谢物的筛选程序。

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A gas chromatography-mass spectrometry (GC-MS)-based screening procedure was developed for the detection of stimulant laxatives and/or their metabolites in human urine after enzymatic cleavage of conjugates followed by extractive methylation. The part of the phase-transfer catalyst remaining in the organic phase was removed by solid-phase extraction on a diol phase. The compounds were separated by capillary GC and identified by computerized MS in the full scan mode. By use of mass chromatography with the ions m/z 305, 290, 335, 320, 365, 350, 311, 326, 271, and 346, the possible presence of stimulant laxatives and/or their metabolites could be indicated. The identity of positive signals in such mass chromatograms was confirmed by comparison of the peaks underlying full mass spectra with the reference spectra. This method allowed the detection of the diphenol laxatives bisacodyl, picosulfate, and phenolphthalein and of the anthraquinone laxatives contained in plant extracts and/or their metabolites in human urine samples. The overall recoveries of the stimulant laxatives and/or their metabolites ranged between 33% and 89% with a coefficient of variation of less than 15%, and the limits of detection ranged between 10 and 25 ng/mL (S/N 3) in the full scan mode. After ingestion of the lowest therapeutic dose of sodium picosulfate, its main metabolite, bisacodyl diphenol, was detectable in urine samples for 72 hours. After ingestion of the lowest therapeutic dose of a senna extract, the main metabolite of sennosides, rhein, was detectable in urine samples for 24 hours. This procedure is part of a systematic toxicological analysis procedure for acidic drugs and poisons with the modification of enzymatic cleavage of conjugates.
机译:建立了一种基于气相色谱-质谱(GC-MS)的筛选方法,用于在酶解结合物后进行提取甲基化后检测人尿中的兴奋性泻药和/或其代谢物。通过在二醇相上进行固相萃取,除去残留在有机相中的部分相转移催化剂。通过毛细管GC分离化合物,并通过计算机MS在全扫描模式下进行鉴定。通过使用离子色谱为m / z 305、290、335、320、365、350、311、326、271和346的质谱,可以表明可能存在刺激性泻药和/或其代谢产物。通过比较完整质谱图下方的峰与参考质谱图,可以确认此类质谱图中阳性信号的身份。该方法可以检测人尿液样品中植物提取物和/或其代谢产物中所含的双酚轻泻药比沙可啶,甲基硫酸盐和酚酞以及蒽醌轻泻药。兴奋性泻药和/或其代谢产物的总回收率在33%至89%之间,变异系数小于15%,检测限在10至25 ng / mL(S / N 3)之间。完整扫描模式。摄入最低治疗剂量的甲基吡啶硫酸钠后,在尿液样本中可检测到其主要代谢物比沙可啶双酚72小时。摄入最低剂量的番泻叶提取物后,在24小时的尿液样本中可检测到番泻苷的主要代谢产物大黄。此过程是对酸性药物和毒物进行系统毒理学分析的一部分,其中修饰了结合物的酶促裂解作用。

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