A new fluorogenic assay for tyrosine-containing peptides.

A new tyrosine-specific LC assay with pre-column fluorogenic derivatization is described for Tyr-Gly as model peptide. o-Hydroxylation of the tyrosine residue with tyrosinase in the presence of ascorbic acid, followed by oxidation to the corresponding quinone by potassium ferricyanide at room temperature and condensation with 1,2-diamino-1,2-diphenylethane in the presence of acetonitrile gave a highly fluorescent species. The resulting fluorescence signal was stable over the investigated period of 5 h and exhibited a linear response curve on a reversed-phase LC system. Under optimized reaction conditions, the lower limit of detection for Tyr-Gly was 200 fmol per injection. Examination of a series of dipeptides (L-Tyr-L-X; X = Gly, Ala, Val, Leu, Phe) showed no significant influence of neighbouring amino acids on the enzymatic hydroxylation by tyrosinase. This and the formation of a highly fluorescent signal for Leu-enkephalin suggests the general feasibility of the approach for the determination of tyrosine-containing peptides.