Deep eutectic solvent extraction of myricetin and antioxidant properties

In this study, a response surface method (RSM) was used to optimise the ultrasonic-assisted deep eutectic solvent (DES) extraction of myricetin from myricetin leaves. The results demonstrated that the DES-5 (choline chloride-oxalic acid) system exhibited better extraction results than the other seven DESs prepared. The optimum extraction conditions for myricetin were a DES-5 system with 19% water content of DES, a liquid-to-solid ratio of 37 : 1 mL g-1, an extraction time of 45 min, and an extraction temperature of 72 degrees C. Under these conditions, the extraction amount of myricetin was 22.47 mg g-1. To optimise the extraction process, the crude myricetin extract was purified, and the optimal conditions were as follows: an AB-8 macroporous adsorption resin was used with an anhydrous ethanol desorption agent. The adsorption rate was 1 BV per h (bed volume per hour), the desorption rate was 1 BV per h, and the desorption capacity was 2 BV (bed volume). The antioxidant properties of the myricetin were also investigated. The results demonstrated that, with an increase in concentration, the scavenging rates of DPPH and (OH)-O-center dot free radicals increased. Compared to Vc, myricetin had a better scavenging ability for DPPH free radicals, whereas purified myricetin had a better antioxidant effect. At the same concentration, the radical-scavenging rate of the (OH)-O-center dot radical was slightly higher in myricetin purified by the macroporous adsorption resin than in Vc, and that of the unpurified myricetin was the smallest. Myricetin was purified using a macroporous adsorption resin to improve its antioxidant properties. In this study, a response surface method (RSM) was used to optimise the ultrasonic-assisted deep eutectic solvent (DES) extraction of myricetin from myricetin leaves.