A novel spectrofluorimetric method for the determination of L ascorbic acid is proposed. It is based on the inhibition of L ascorbic acid on the formation of 2,3 diaminophenazine, which is an oxidation product of ...A novel spectrofluorimetric method for the determination of L ascorbic acid is proposed. It is based on the inhibition of L ascorbic acid on the formation of 2,3 diaminophenazine, which is an oxidation product of o phenylenediamine catalyzed by laccase .The fluorescence (at λ ex /λ em =464 nm /530 nnm) was enhanced strongly in the presence of organic media . The mechanism of o phenylenediamine oxidation reaction catalyzed by laccase in the presence of L ascorbic acid is discussed .L ascorbic acid is determined in the ethanol, 1,4 dioxane and acetone over the linear range of 4.0×10 -7 ~1.2×10 -4 mol/L, 4.0×10 -7 ~ 8.0×10 -5 mol/L and 4.0×10 -7 ~1.0×10 -4 mol/L with a detection limit of 1.20×10 -8 mol/L,1.19×10 -8 mol/L and 1.24×10 -8 mol/L, respectively. The method has been successfully applied to the simple and rapid determination of L ascorbic acid in pharmaceuticals and milk powder.展开更多
文摘A novel spectrofluorimetric method for the determination of L ascorbic acid is proposed. It is based on the inhibition of L ascorbic acid on the formation of 2,3 diaminophenazine, which is an oxidation product of o phenylenediamine catalyzed by laccase .The fluorescence (at λ ex /λ em =464 nm /530 nnm) was enhanced strongly in the presence of organic media . The mechanism of o phenylenediamine oxidation reaction catalyzed by laccase in the presence of L ascorbic acid is discussed .L ascorbic acid is determined in the ethanol, 1,4 dioxane and acetone over the linear range of 4.0×10 -7 ~1.2×10 -4 mol/L, 4.0×10 -7 ~ 8.0×10 -5 mol/L and 4.0×10 -7 ~1.0×10 -4 mol/L with a detection limit of 1.20×10 -8 mol/L,1.19×10 -8 mol/L and 1.24×10 -8 mol/L, respectively. The method has been successfully applied to the simple and rapid determination of L ascorbic acid in pharmaceuticals and milk powder.
