The effect of substrate partitioning on the kinetics of enzymes acting in reverse micelles

Abstract

A theoretical model for the expression of enzymic activity in reverse micelles previously developed [Bru, Sanchez-Ferrer and Garcia-Carmona (1989) Biochem. J. 259, 355-361] was extended in the present work. The substrate concentration in each reverse-micelle phase (free water, bound water and surfactant apolar tails) and the organic solvent was expressed as a function of the total substrate concentration, taking into account its partition coefficients, that is, partitioning of the substrate in a multiphasic system. In each phase the enzyme expresses a catalytic constant and a Km. Thus the whole reaction rate is the addition of the particular rates expressed in each domain. this model was compared with that developed for a biphasic system [Levashov, Klyachko, Pantin, Khmelnitski and Martinek (1980) Bioorg. Khim. 6 929-943] by fitting the experimental results obtained with mushroom tyrosinase (working on both 4-t-butylcatechol and 4-methylcatechol) to the two models. The parameters which characterize reverse micelles, .omega.0 (water/surfactant molar ratio) and .theta. (fraction of water) were investigated. The .omega.0 profile was shown to be hyperbolic for both substrates. Activity towards 4-t-butylcatechol decreases as .theta. increases, this observation being attributable to a dilution of the substrate. A Km of 7.8 M for 4-t-butylcatechol could be calculated on the basis of the biphasic model, whereas it was 13.5 mM when calculating on the basis of our model. a new parameter, .rho. (= [substrate]/.theta.), was defined to characterize those substrates that mainly solubilize in the reverse micelle (''micellar substrates'').