SEGMENTAL MOTION IN CATALYSIS - INVESTIGATION OF A HYDROGEN-BOND CRITICAL FOR LOOP CLOSURE IN THE REACTION OF TRIOSEPHOSPHATE ISOMERASE

A residue essential for proper closure of the active-site loop in the reaction catalyzed by triosephosphate isomerase is tyrosine-208, the hydroxyl group of which forms a hydrogen bond with the amide nitrogen of alanine-176, a component of the loop. Both residues are conserved, and mutagenesis of the tyrosine to phenylalanine results in a 2000-fold drop in the catalytic activity (k(cat)/K(m)) of the enzyme compared to the wild-type isomerase. The nature of the closure process has been elucidated from both viscosity dependence and primary isotope effects. The reaction catalyzed by the mutant enzyme shows a viscosity dependence using glycerol as the viscosogen. This dependence can be attributed to the rate-limiting motion of the active-site loop between the "open" and the "closed" conformations. Furthermore, a large primary isotope effect is observed with [1-H-2]dihydroxyacetone phosphate as substrate [(k(cat)/K(m))H/k(cat)/K(m))D = 6 +/- 1]. The range of isotopic experiments that were earlier used to delineate the energetics of the wild-type isomerase has provided the free energy profile of the mutant enzyme. Comparison of the energetics of the wild-type and mutant enzymes shows that only the transition states flanking the enediol intermediate have been substantially affected. The results suggest either that loop closure and deprotonation are coupled and occur in the same rate-limiting step or that these two processes happen sequentially but interdependently. This finding is consistent with structural information that indicates that the catalytic base glutamate-165 moves 2 angstrom toward the substrate upon loop closure. The motion of the mobile loop of triosephosphate isomerase is therefore linked to substrate deprotonation by the catalytic base glutamate-165.