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采用液相色谱-荧光检测法分离和测定人尿中的 11 种标记蝶呤。

Separation and determination of 11 marker pteridines in human urine by liquid chromatography and fluorimetric detection.

机构信息

Department of Analytical Chemistry, University of Extremadura, Badajoz, Spain.

出版信息

J Sep Sci. 2011 Jun;34(11):1283-92. doi: 10.1002/jssc.201000900. Epub 2011 Apr 20.

Abstract

A simple liquid chromatographic method has been developed to achieve the complete separation and determination of a wide range of pteridinic compounds and creatinine (CREA) in urine samples, in just one run. The influences of mobile phase composition and buffer pH have been studied. The optimized mobile phase was composed of a Tris-HCl buffer (15 mmol/L) at pH 6.10 solution (eluent A) and a Tris-HCl buffer (15 mmol/L) at pH 6.40 solution (eluent B), in gradient mode. Analytes were determined by fluorimetric detection, exciting at 272 nm, and measuring the fluorescence emission at three wavelengths, 410, 445 and 465 nm. CREA, as a reference of metabolites excretion in urine, was determined by photometric detection at 230 nm. Pteridines detection limits varied from 0.2 to 6.1 ng/mL, and 0.2 g/mL for CREA. Calculated precision values expressed as RSD (%) varied from 1.1 to 5.9. Two different oxidation procedures for urine samples were optimized. The neopterin/biopterin ratios found were 0.98 and 0.86 for adults and children, respectively, by means of the alkaline iodide/iodine oxidation and 0.45 and 0.57 using neutral KMnO(4) oxidation.

摘要

已开发出一种简单的液相色谱方法,可在一次运行中实现尿液样品中多种蝶啶化合物和肌酸酐(CREA)的完全分离和测定。研究了流动相组成和缓冲液 pH 值的影响。优化的流动相由 Tris-HCl 缓冲液(15 mmol/L)在 pH 6.10 溶液(洗脱剂 A)和 Tris-HCl 缓冲液(15 mmol/L)在 pH 6.40 溶液(洗脱剂 B)组成,采用梯度模式。采用荧光检测法,在 272nm 激发波长下,在 410nm、445nm 和 465nm 三个波长下测量荧光发射,测定 CREA 等分析物。CREA 作为尿液中代谢物排泄的参考物,在 230nm 处采用分光光度法测定。蝶啶类物质的检测限为 0.2 至 6.1ng/mL,CREA 的检测限为 0.2g/mL。表示为 RSD(%)的计算精密度值变化范围为 1.1 至 5.9。优化了两种不同的尿液样品氧化程序。通过碱性碘化钾/碘氧化,成人和儿童的新蝶呤/生物蝶呤比值分别为 0.98 和 0.86,而使用中性 KMnO4 氧化,该比值分别为 0.45 和 0.57。

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