Your search keyword '"Garcia-Molina M"' showing total 2 results

1. Melanogenesis inhibition due to NADH.

Author

Garcia-Molina F, Munoz-Munoz JL, Garcia-Molina M, Garcia-Ruiz PA, Tudela J, García-Cánovas F, and Rodriguez-Lopez JN

Subjects

Agaricales chemistry, Agaricales physiology, Benzoquinones, Dihydroxyphenylalanine analogs & derivatives, Fungal Proteins, Indoles metabolism, Kinetics, Melanins metabolism, Monophenol Monooxygenase chemistry, Oxidation-Reduction, Substrate Specificity, Indoles antagonists & inhibitors, Monophenol Monooxygenase metabolism, NAD pharmacology

Abstract

The effect of NADH on melanogenesis under aerobic conditions involves three types of reaction: (a) acting as tyrosinase substrate (a competitive substrate of L-tyrosine and L-DOPA), (b) irreversible inactivation acting as a suicide substrate of tyrosinase, and (c) non-enzymatic reduction of o-dopaquinone by NADH. Under anaerobic conditions, NADH irreversibly inhibits the enzymatic forms met-tyrosinase and deoxy-tyrosinase. In this paper, we kinetically characterize this coenzyme as it acts as a tyrosinase suicide substrate and propose a kinetic mechanism to explain its oxidation by tyrosinase. In addition, the compound is characterized as an irreversible inhibitor of met-tyrosinase and deoxy-tyrosinase.

Published

2010

2. Kinetic characterization of the oxidation of carbidopa and benserazide by tyrosinase and peroxidase.

Author

Munoz-Munoz JL, Garcia-Molina F, Garcia-Molina M, Tudela J, García-Cánovas F, and Rodriguez-Lopez JN

Subjects

Kinetics, Oxidation-Reduction, Spectrophotometry, Ultraviolet, Benserazide metabolism, Carbidopa metabolism, Monophenol Monooxygenase metabolism, Peroxidases metabolism

Abstract

Carbidopa and benserazide have been described as inhibitors of dopa decarboxylase and both have been used in the treatment of Parkinson's disease. Because of their chemical structure as polyphenols, these compounds can behave as substrates of tyrosinase and peroxidase. We demonstrate that these enzymes oxidize both substrates. Since o-quinones are unstable, a chronometric method for enzymatic initial rate determinations was used based on measurements of the lag period in the presence of micromolar concentrations of ascorbic acid to kinetically characterize these substrates. In the case of tyrosinase, the values of the Michaelis constant for both substrates were greater than those described for dopa, although the catalytic constants were lower, probably due to the greater size of the substitute group in carbon 1. As regards peroxidase, the saturation of the enzyme by both substrates is possible, however this effect does not occur with the isomers of dopa. The distance of the charges from the benzene ring may enable the ring to approach the iron of the active site and, therefore, act.

Published

2009