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使用电子捕获负离子质谱法对酸性色氨酸代谢物进行定量的五氟苄基化方法。

Pentafluorobenzylation method for quantification of acidic tryptophan metabolites using electron capture negative ion mass spectrometry.

作者信息

Naritsin D B, Boni R L, Markey S P

机构信息

Section on Analytical Biochemistry, National Institute of Mental Health, Bethesda, Maryland 20892-1262, USA.

出版信息

Anal Chem. 1995 Mar 1;67(5):863-70. doi: 10.1021/ac00101a012.

Abstract

An improved pentafluorobenzylation method was developed for derivatization of L-tryptophan and its acidic metabolites (L-kynurenine, kynurenic acid, anthranilic acid, xanthurenic acid, 3-hydroxyanthranilic acid, picolinic acid, quinolinic acid) present at trace levels in aqueous samples. This method employs lyophilization of aqueous samples in the presence of excess tetrabutylammonium hydrogen sulfate, followed by base-catalyzed anhydrous pentafluorobenzylation. A comparison with other published methods shows the advantage of this modification for the derivatization of kynurenine metabolites. The derivatives were analyzed by gas chromatography/electron capture negative ion mass spectrometry (GC/ECNI-MS) or liquid chromatography/particle beam/ECNI-MS (LC/ECNI-MS). The detection limits for injected standards are in the femtogram range by GC/ECNI-MS and in the low picogram range by LC/ECNI-MS. GC/ECNIMS is 3.6 (xanthurenic acid) to 66 (quinolinic acid) times more sensitive than LC/ECNI-MS. The simultaneous determination of two neuroactive metabolites, quinolinic and kynurenic acids, in culture medium is presented. The minimum measurable concentrations of these metabolites in 100 microL of culture medium are 0.11 nM for quinolinic acid and 0.21 nM for kynurenic acid.

摘要

开发了一种改进的五氟苄基化方法,用于衍生化水性样品中痕量存在的L-色氨酸及其酸性代谢物(L-犬尿氨酸、犬尿酸、邻氨基苯甲酸、黄尿酸、3-羟基邻氨基苯甲酸、吡啶甲酸、喹啉酸)。该方法采用在过量硫酸氢四丁铵存在下对水性样品进行冻干,然后进行碱催化的无水五氟苄基化。与其他已发表方法的比较表明了这种改进对于犬尿氨酸代谢物衍生化的优势。衍生物通过气相色谱/电子捕获负离子质谱(GC/ECNI-MS)或液相色谱/粒子束/ECNI-MS(LC/ECNI-MS)进行分析。注入标准品的检测限通过GC/ECNI-MS在飞克范围内,通过LC/ECNI-MS在低皮克范围内。GC/ECNIMS的灵敏度比LC/ECNI-MS高3.6倍(黄尿酸)至66倍(喹啉酸)。本文介绍了在培养基中同时测定两种神经活性代谢物喹啉酸和犬尿酸的方法。在100微升培养基中,这些代谢物的最低可测浓度对于喹啉酸为0.11 nM,对于犬尿酸为0.21 nM。

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