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首页> 外文期刊>Journal of forensic sciences. >Aqueous phase hexylchloroformate derivatization and solid phase microextraction: determination of benzoylecgonine in urine by gas chromatography-quadrupole ion trap mass spectrometry.
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Aqueous phase hexylchloroformate derivatization and solid phase microextraction: determination of benzoylecgonine in urine by gas chromatography-quadrupole ion trap mass spectrometry.

机译:水相氯甲酸甲酸酯的衍生化和固相微萃取:气相色谱-四极杆离子阱质谱法测定尿液中的苯甲酰芽子碱。

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摘要

A derivatization/solid phase microextraction (SPME) method for the determination of benzoylecgonine in urine was developed. The derivatization is conducted directly in 1 mL of urine while sonicating for 3 min with 12 microL of hexyl chloroformate and 70 microL of a mixture containing acetonitrile:water:hexanol:2-dimethylaminopyridine (5:2:2:1 v/v), yielding benzoylecgonine hexyl ester (BHE) as the product. After the 3 min period, an aliquot of 250 microL is transferred to a vial for SPME. After the desired extraction time the 100 microns polydimethylsiloxane SPME fiber was transferred to the GC-MS for separation and analysis with a quadrupole ion trap mass spectrometer. The hexyl chloroformate derivatization and SPME procedures were optimized for compatibility and sensitivity. The method was found linear for 0.10 to 20.0 micrograms/mL (r2 = 0.999) of benzoylecgonine in urine using benzoylecgonine-d3 as an internal standard (1.5 micrograms/mL). Intra-day precisions were 8.8 and 6.8% RSD for 0.30 microgram/mL and 17 micrograms/mL benzoylecgonine standards in urine (n = 6), respectively. Inter-day precision (n = 3) were < or = 3.3% RSD, indicating good reproducibility. A detection limit of 0.03 microgram/mL (S/N = 3) was achieved, thus making the SPME method a simplified alternative to SPE for GC-MS confirmation after EMIT tests for benzoylecgonine which have a cutoff of 0.30 microgram/mL. Quantitative results by SPME and SPE of two clinical urine specimens known positive for cocaine by EMIT were in excellent agreement. Benzoylecgonine was detected by the derivatization/SPME method in 22 out of 22 other urine specimens known positive for cocaine.
机译:建立了衍生化/固相微萃取(SPME)法测定尿液中苯甲酰芽子碱的方法。直接在1 mL尿液中进行衍生化,同时与12微升氯甲酸己酯和70微升含乙腈:水:己醇:2-二甲基氨基吡啶(5:2:2:1 v / v)的混合物超声处理3分钟,产生苯甲酰基芽子碱己酯(BHE)作为产物。 3分钟后,将250微升的等分试样转移至用于SPME的小瓶中。在所需的萃取时间后,将100微米的聚二甲基硅氧烷SPME纤维转移到GC-MS中,以使用四极离子阱质谱仪进行分离和分析。氯甲酸己酯的衍生化和SPME程序进行了优化的兼容性和灵敏度。使用苯甲酰芽子碱-d3作为内标物(1.5微克/ mL),尿液中苯甲酰芽子碱的线性范围为0.10至20.0微克/ mL(r2 = 0.999)。尿液中苯甲酰芽子碱的标准浓度为0.30微克/毫升和17微克/毫升的日内精密度分别为8.8和6.8%(n = 6)。日间精度(n = 3)≤RSD = 3.3%,表明可重复性好。达到了0.03微克/ mL(S / N = 3)的检测限,因此使SPME方法成为SPE的简化替代方法,用于EMIT测试苯甲酰芽子碱的标准品,其临界值为0.30微克/ mL,用于GC-MS确认。 SPME和SPE对EMIT已知可卡因呈阳性的两个临床尿液标本的定量结果非常吻合。通过衍生化/ SPME方法在已知可卡因呈阳性的其他22个尿液样本中的22个中检测到苯甲酰吗啡。

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