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使用固定化酶作为柱后反应器并结合电化学检测的生物多胺高效液相色谱法。

High performance liquid chromatography of biological polyamines using immobilized enzyme as post-column reactor followed by electrochemical detection.

作者信息

Watanabe N, Asano M, Yamamoto K, Nagatsu T, Matsumoto T, Fujita K

机构信息

Department of Industrial Chemistry, Faculty of Engineering, University of Tokyo, Japan.

出版信息

Biomed Chromatogr. 1989 Sep;3(5):187-91. doi: 10.1002/bmc.1130030502.

Abstract

A novel analytical method for biological polyamines (putrescine, spermidine and spermine) was developed. Polyamines were separated by ion-pair reversed phase chromatography using a polymer-based octadecyl bonded column. A polyamine oxidase immobilized column worked effectively as a post-column reactor to convert polyamines to hydrogen peroxide which was eventually detected by electrochemical oxidation on platinum electrode. This method required neither tedious derivatization nor gradient elution, permitting us to perform simple and rapid analysis of polyamines. The detection limits were 0.3, 0.6, and 4 pmol injected for putrescine, spermidine, and spermine, respectively with a linear range of two to three orders of magnitude. Chromatograms obtained with samples from human urine and rat brain homogenates demonstrated the high sensitivity and selectivity of the method.

摘要

开发了一种用于生物多胺(腐胺、亚精胺和精胺)的新型分析方法。使用基于聚合物的十八烷基键合柱通过离子对反相色谱法分离多胺。固定有多胺氧化酶的柱子作为柱后反应器有效地将多胺转化为过氧化氢,最终通过铂电极上的电化学氧化进行检测。该方法既不需要繁琐的衍生化也不需要梯度洗脱,使我们能够对多胺进行简单快速的分析。腐胺、亚精胺和精胺的检测限分别为注入0.3、0.6和4 pmol,线性范围为两到三个数量级。用人尿和大鼠脑匀浆样品获得的色谱图证明了该方法的高灵敏度和选择性。

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