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Unraveling the Antioxidant Activity of 2R,3R-dihydroquercetin

INTERNATIONAL JOURNAL OF MOLECULAR SCIENCES [2023]
Yaping Xu, Zhengwen Li, Yue Wang, Chujie Li, Ming Zhang, Haiming Chen, Wenxue Chen, Qiuping Zhong, Jianfei Pei, Weijun Chen, Guido R. M. M. Haenen, Mohamed Moalin
ABSTRACT

It has been reported that in an oxidative environment, the flavonoid2R,3R-dihydroquercetin (2R,3R-DHQ) oxidizes into a product that rearranges to form quercetin. As quercetin is a very potent antioxidant, much better than2R,3R-DHQ, this would be an intriguing form of targeting the antioxidant quercetin. The aim of the present study is to further elaborate on this targeting. We can confirm the previous observation that2R,3R-DHQ is oxidized by horseradish peroxidase (HRP), with H2O2as the oxidant. However, HPLC analysis revealed that no quercetin was formed, but instead an unstable oxidation product. The inclusion of glutathione (GSH) during the oxidation process resulted in the formation of a2R,3R-DHQ-GSH adduct, as was identified using HPLC with IT-TOF/MS detection. GSH adducts appeared on the B-ring of the2R,3R-DHQ quinone, indicating that during oxidation, the B-ring is oxidized from a catechol to form a quinone group. Ascorbate could reduce the quinone back to2R,3R-DHQ. No2S,3R-DHQ was detected after the reduction by ascorbate, indicating that a possible epimerization of2R,3R-DHQ quinone to2S,3R-DHQ quinone does not occur. The fact that no epimerization of the oxidized product of2R,3R-DHQ is observed, and that GSH adducts the oxidized product of2R,3R-DHQ on the B-ring, led us to conclude that the redox-modulating activity of2R,3R-DHQ quinone resides in its B-ring. This could be confirmed by chemical calculation. Apparently, the administration of2R,3R-DHQ in an oxidative environment does not result in ‘biotargeting’ quercetin.Keywords:2R,3R-dihydroquercetin;redox modulation;quercetin;quinone;epimerization

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