Fluorometric determination of hydrogen peroxide using resorufin and peroxidase

Abstract

A fluorometric method for the determination of hydrogen peroxide using resorufin as a substrate for peroxidase is described. Two procedures were developed for the determination of hydrogen peroxide. One involves the addition of hydrogen peroxide sample to a solution of peroxidase and resorufin in phosphate buffer, pH 6.4. Fluorescence measurements are performed before and after hydrogen peroxide addition. The within-run CVs for final concentrations of hydrogen peroxide of 200 and 40 nmol/liter were 1.7 and 7.6%, respectively, and the limit of quantitation was 9 nmol/liter. The second procedure, in which the initial reaction of hydrogen peroxide with resorufin is performed in citrate buffer at pH 4.5, and then the fluorescence is measured after the pH is adjusted to 9.2 with borate buffer, has a limit of quantitation of 4.4 nmol/liter with a within-run CV of 6.5% for a final hydrogen peroxide concentration of 20 nmol/liter. The method is linear at least up to 1 μmol/liter.