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The Scopoletin-HRP Fluorimetric Determination of H2O2 in Seawaters—A Plea for the Two-Stage Protocol

机译:水溶素-HRP荧光测定海洋水域中H2O2的荧光测定 - 用于两阶段方案的请求

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摘要

A single solution protocol has been widely used for the fluorimetric determination of H2O2 in natural waters by its bleaching of the fluorescing scopoletin in the presence of the enzyme horseradish peroxidase (HRP). In this protocol, the reaction between scopoletin and H2O2 in the sample and the subsequent internal additions, and the measurements of the fluorescence are all carried out at a single pH in a fluorometer cell. It is found that this protocol is prone to four sources of possible error. The variability in the reaction stoichiometry between scopoletin and H2O2 in the presence of varying amounts of excess scopoletin, the effect of pH on the rate of reaction between scopoletin and H2O2, the photobleaching of scopoletin, and the de-activation of HRP. These possible sources of error can be circumvented in a two-stage protocol in which the reaction between H2O2 and scopoletin is carried out immediately upon sampling at a pH of 7, and the measurement of the fluorescence is carried out later on at a pH of 9. It should be the protocol of choice. Furthermore, in the two-stage protocol, after the initial reaction between H2O2 and scopoletin, the sample may be stored at room temperature for six days and at 4 °C for at least a month before its fluorescence is measured. This option can significantly reduce the logistics in the field.
机译:通过在酶辣根过氧化物酶(HRP)存在下,通过漂白荧光微调蛋白的漂白,广泛用于荧光测定天然水中的荧光测定。在该方案中,样品中Scopoletin和H 2 O 2之间的反应和随后的内部添加,以及荧光的测量全部在荧光计细胞中的单个pH下进行。发现该协议容易出现四种可能误差的源。在不同量的过量水循环蛋白存在下,Scopoletin和H 2 O 2之间的反应化学计量的变异性,pH对水溶素和H 2 O 2之间的反应速率,Scopoletin的光漂白的作用,以及HRP的去活化。这些可能的误差源可以在两级方案中避免,其中在在pH的pH下采样时立即进行H 2 O 2和Scopoletin之间的反应,并且荧光的测量在稍后在9的pH下进行。它应该是选择的协议。此外,在两级方案中,在H 2 O 2和Scopoletin之间的初始反应之后,样品可以在室温下储存六天,在测量其荧光之前至少一个月在4℃下储存六天。此选项可以显着减少现场物流。

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