汞膜电极吸附溶出伏安法测定次黄嘌呤中的黄嘌呤。

Analytical Chemistry Insights Pub Date : 2014-06-09 eCollection Date: 2014-01-01 DOI:10.4137/ACI.S14712
Percio Augusto Mardini Farias, Arnaldo Aguiar Castro
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引用次数: 2

摘要

描述了一种在亚微摩尔浓度的次黄嘌呤存在下测定黄嘌呤的溶出方法。该方法是基于在薄膜汞电极上控制吸附积累,然后对表面物质进行快速线性扫描伏安测量。最佳实验条件为:以1.0 × 10(-3) mol L(-1) NaOH溶液为支撑电解质,黄嘌呤的积累电位为0.00 V,次黄嘌呤-铜的积累电位为-0.50 V,线性扫描速率为200 mV秒(-1)。黄嘌呤的响应在20-140 ppb的浓度范围内呈线性。积累时间为30min,检出限为36ppt (2.3 × 10(-10) mol L(-1))。在次黄嘌呤、铜和其他金属、尿酸和其他氮化碱存在的情况下测定黄嘌呤的适当条件也进行了研究。该方法的实用性通过与次黄嘌呤、尿酸、氮化碱基、ATP和ssDNA相关的黄嘌呤的存在得到证明。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Determination of xanthine in the presence of hypoxanthine by adsorptive stripping voltammetry at the mercury film electrode.

Determination of xanthine in the presence of hypoxanthine by adsorptive stripping voltammetry at the mercury film electrode.

Determination of xanthine in the presence of hypoxanthine by adsorptive stripping voltammetry at the mercury film electrode.

Determination of xanthine in the presence of hypoxanthine by adsorptive stripping voltammetry at the mercury film electrode.

A stripping method for the determination of xanthine in the presence of hypoxanthine at the submicromolar concentration levels is described. The method is based on controlled adsorptive accumulation at the thin-film mercury electrode followed by a fast linear scan voltammetric measurement of the surface species. Optimum experimental conditions were found to be the use of 1.0 × 10(-3) mol L(-1) NaOH solution as supporting electrolyte, an accumulation potential of 0.00 V for xanthine and -0.50 V for hypoxanthine-copper, and a linear scan rate of 200 mV second(-1). The response of xanthine is linear over the concentration ranges of 20-140 ppb. For an accumulation time of 30 minutes, the detection limit was found to be 36 ppt (2.3 × 10(-10) mol L(-1)). Adequate conditions for measuring the xanthine in the presence of hypoxanthine, copper and other metals, uric acid, and other nitrogenated bases were also investigated. The utility of the method is demonstrated by the presence of xanthine associated with hypoxanthine, uric acid, nitrogenated bases, ATP, and ssDNA.

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