[No authors listed]
Tetrahydrobiopterin (BHâ) is required for NO synthesis and inhibition of superoxide release from endothelial NO synthase. Clinical trials using BHâ to treat endothelial dysfunction have produced mixed results. Poor outcomes may be explained by the rapid systemic and cellular oxidation of BHâ. One of the oxidation products of BHâ, 7,8-dihydrobiopterin (7,8-BHâ), is recycled back to BHâ by dihydrofolate reductase (DHFR). This enzyme is ubiquitously distributed and shows a wide range of activity depending on species-specific factors and cell type. Information about the kinetics and efficiency of BH4 recycling in human endothelial cells receiving BHâ treatment is lacking. To characterize this reaction, we applied a novel multielectrode coulometric HPLC method that enabled the direct quantification of 7,8-BHâ and BHâ, which is not possible with fluorescence-based methodologies. We found that basal untreated BHâ and 7,8-BHâ concentrations in human endothelial cells (ECs) are lower than in bovine and murine endothelioma cells. Treatment of human ECs with BHâ transiently increased intracellular BHâ while accumulating the more stable 7,8-BHâ. This was different from bovine or murine ECs, which resulted in preferential BHâ increase. Using BHâ diastereomers, 6S-BHâ and 6R-BHâ, the narrow contribution of enzymatic DHFR recycling to total intracellular BHâ was demonstrated. Reduction of 7,8-BHâ to BHâ occurs at very slow rates in cells and needs supraphysiological levels of 7,8-BHâ, indicating this reaction is kinetically limited. Activity assays verified that human DHFR has very low affinity for 7,8-BHâ (DHF
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