INFLUENCE OF ELECTROSTATIC FACTORS AND INTERACTIONS WITH SOLVENT ON THE RATE OF EXCITED-STATE PROTON-TRANSFER FOR 2-NAPHTHOL DERIVATIVES BOUND COVALENTLY TO SELECTED SITES OF PROTEINS

2-Naphthol-6-sulphonic acid (NSOH) was bound to bovine serum albumin ( BSA) by a sulphonamide bond. Carboxyl or amino groups of the protein w ere then modified by a neutral group which induced variation of the gr ound state pK(a) and excited state pK(a) values of the NSOH groups bo und to the protein. The rate constants (k(pt)) of excited state proton transfer (ESPT) in NSOH groups bound to BSA were determined by steady state fluorescence spectroscopy. The dependence of log k(pt) on log K (a) for BSA-NSOH conjugates was fitted to a modified Bronsted relatio n. This plot was treated as a reference curve for comparison with anal ogous data for NSOH groups bound to other protein samples. Deviations from this plot were explained by kinetic isotope effects. It is postul ated that certain essential features of the ESPT mechanism are varied as a consequence of changes in parameters of the microenvironment of t he proton donor, such as the optical dielectric permittivity and the d istance to other charged groups of the protein. Thus when the fluoroph ore is bound preferentially to the surface of the protein globule by a spacer (approximately 2.5 angstrom) the diffusion of water as a proto n acceptor is the rate-limiting step in ESPT. When the same fluorophor e is bound to the surface of the macromolecule by a sulphonamide bond anchored directly to an amino group of the protein, partition of a pro ton is the rate-determining step leading to a ''negative'' isotope eff ect and a low rate of ESPT. When the fluorophore is bound inside the p rotein molecule, proton transfer through a chain of preformed hydrogen bonds is responsible for a much higher rate of ESPT than in the other samples.