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用于直接浸入式固相微萃取的纤维上衍生化。第二部分。用五氟苯甲酰氯对苯丙胺进行酰化用于尿液分析。

On-fiber derivatization for direct immersion solid-phase microextraction. Part II. Acylation of amphetamine with pentafluorobenzoyl chloride for urine analysis.

作者信息

Koster E H M, Bruins C H P, de Jong G J

机构信息

Department of Pharmaceutical Analysis, University Centre for Pharmacy, AD Groningen, The Netherlands.

出版信息

Analyst. 2002 May;127(5):598-602. doi: 10.1039/b110590f.

DOI:10.1039/b110590f
PMID:12081035
Abstract

On-fiber derivatization was used for solid-phase microextraction (SPME) in order to increase the detectability and extractability of drugs in biological samples. Amphetamine, which was used as a model compound, was derivatized with pentafluorobenzoyl chloride (PFBCl) and subjected to gas chromatography with electron capture or mass spectrometric detection. Extraction was performed by direct immersion of a 100 microm polydimethylsiloxane-coated fiber into buffered human urine. On-fiber derivatization was performed either after or simultaneously with extraction. The former procedure gave cleaner chromatograms but the latter turned out to be superior with respect to linearity and repeatability. For the on-fiber derivatization of amphetamine an excess of reagent is required. Because a considerable part of the PFBCl loaded on to the fiber is used up by reaction with matrix compounds and water, a reagent loading time of 5 min was needed to obtain a linear range (r = 0.9756) from 250 pg mL(-1) to 15 ng mL(-1). Due to an interfering matrix compound, the limit of detection was also found to be dependent on the reagent loading time, i.e., the limit of detection for a PFBCl loading time of 5 min is 250 pg mL(-1) whereas that for a 1 min loading time it is 100 pg mL(-1). The relative standard deviation (n = 7) of the method was about 11% at an amphetamine concentration of 1 ng mL(-1). The applicability of the method for the determination of drugs in biological samples is shown.

摘要

为了提高生物样品中药物的可检测性和可萃取性,采用纤维上衍生化进行固相微萃取(SPME)。以苯丙胺作为模型化合物,用五氟苯甲酰氯(PFBCl)进行衍生化,然后进行气相色谱分析,并采用电子捕获或质谱检测。通过将100微米聚二甲基硅氧烷涂层纤维直接浸入缓冲的人尿中进行萃取。纤维上衍生化在萃取后或与萃取同时进行。前一种方法得到的色谱图更干净,但后一种方法在线性和重复性方面表现更优。对于苯丙胺的纤维上衍生化,需要过量的试剂。由于负载在纤维上的相当一部分PFBCl会与基质化合物和水反应而消耗掉,因此需要5分钟的试剂负载时间才能获得250 pg mL(-1)至15 ng mL(-1)的线性范围(r = 0.9756)。由于存在干扰基质化合物,检测限也被发现取决于试剂负载时间,即PFBCl负载时间为5分钟时的检测限为250 pg mL(-1),而负载时间为1分钟时的检测限为100 pg mL(-1)。在苯丙胺浓度为1 ng mL(-1)时,该方法的相对标准偏差(n = 7)约为11%。展示了该方法在生物样品中药物测定方面的适用性。

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