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利用同位素稀释串联质谱法对人尿液中的石房蛤毒素和新石房蛤毒素进行定量分析。

Quantification of saxitoxin and neosaxitoxin in human urine utilizing isotope dilution tandem mass spectrometry.

作者信息

Johnson Rudolph C, Zhou Yingtao, Statler Kristen, Thomas Jerry, Cox Frederick, Hall Sherwood, Barr John R

机构信息

Division of Laboratory Sciences, Centers for Disease Control and Prevention, 4770 Buford Highway, MS F44, Atlanta, Georgia 30341, USA.

出版信息

J Anal Toxicol. 2009 Jan-Feb;33(1):8-14. doi: 10.1093/jat/33.1.8.

Abstract

Saxitoxin and neosaxitoxin are potent neurotoxins that can cause paralytic shellfish poisoning when consumed. A new assay is presented here to quantify saxitoxin (STX) and neosaxitoxin (NEO) in human urine samples. Sample preparation of 500-microL samples included the use of weak-cation-exchange solid-phase extraction in a multiplexed 96-well format. Extracts were preconcentrated and analyzed via 10-min hydrophilic interaction liquid chromatography followed by electrospray ionization. Protonated molecular ions were quantified via multiple reaction monitoring mode in a Qtrap mass spectrometer. The method uses novel 15N7-isotopically enriched STX and NEO internal standards. Method validation included the characterization of two enriched urine pools. The lowest reportable limits for STX and NEO were 4.80 and 10.1 ng/mL, respectively, using both quantification and confirmation ions. These two toxins were not detected in a reference range of humans who consumed seafood in the preceding 72 h, suggesting that few false positives would occur when trying to identify people exposed to STX or NEO.

摘要

石房蛤毒素和新石房蛤毒素是强效神经毒素,食用后可导致麻痹性贝类中毒。本文介绍了一种新的检测方法,用于定量检测人类尿液样本中的石房蛤毒素(STX)和新石房蛤毒素(NEO)。500微升样本的制备包括在96孔多重格式中使用弱阳离子交换固相萃取。提取物经预浓缩后,通过10分钟的亲水作用液相色谱,然后进行电喷雾电离分析。在Qtrap质谱仪中,通过多反应监测模式对质子化分子离子进行定量。该方法使用新型的15N7同位素富集的STX和NEO内标。方法验证包括对两个富集尿液池的表征。使用定量和确证离子时,STX和NEO的最低报告限分别为4.80和10.1纳克/毫升。在前72小时内食用过海鲜的人群参考范围内未检测到这两种毒素,这表明在试图识别接触过STX或NEO的人群时,很少会出现假阳性结果。

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