Inverse enzyme isotope effects in human purine nucleoside phosphorylase with heavy asparagine labels

<p id="d2054394e199">Enzymes achieve catalytic efficiency by optimizing contacts between reactants and catalytic site amino acids. The transition state forms rarely, with a lifetime of a few femtoseconds. Femtosecond motions required for transition state formation are investigated with heavy enzymes containing ²H, ¹³C, and ¹⁵N amino acids to alter bond vibrational modes. Asparagine is a critical amino acid at the catalytic site of human purine nucleoside phosphorylase (PNP). PNP with heavy asparagine, or with all heavy amino acids except asparagine, yields PNPs more efficient at forming the transition state. Computational chemistry reveals that essential catalytic site contacts become more frequently optimized in the labeled enzymes than in the normal enzyme. Heavy enzymes provide unprecedented detail for understanding enzymatic catalysis. </p><p class="first" id="d2054394e211">Transition path-sampling calculations with several enzymes have indicated that local catalytic site femtosecond motions are linked to transition state barrier crossing. Experimentally, femtosecond motions can be perturbed by labeling the protein with amino acids containing ¹³C, ¹⁵N, and nonexchangeable ²H. A slowed chemical step at the catalytic site with variable effects on steady-state kinetics is usually observed for heavy enzymes. Heavy human purine nucleoside phosphorylase (PNP) is slowed significantly ( <i>k</i> _chem _light/ <i>k</i> _chem _heavy = 1.36). An asparagine (Asn243) at the catalytic site is involved in purine leaving-group activation in the PNP catalytic mechanism. In a PNP produced with isotopically heavy asparagines, the chemical step is faster ( <i>k</i> _chem _light/ <i>k</i> _chem _heavy = 0.78). When all amino acids in PNP are heavy except for the asparagines, the chemical step is also faster ( <i>k</i> _chem _light/ <i>k</i> _chem _heavy = 0.71). Substrate-trapping experiments provided independent confirmation of improved catalysis in these constructs. Transition path-sampling analysis of these partially labeled PNPs indicate altered femtosecond catalytic site motions with improved Asn243 interactions to the purine leaving group. Altered transition state barrier recrossing has been proposed as an explanation for heavy-PNP isotope effects but is incompatible with these isotope effects. Rate-limiting product release governs steady-state kinetics in this enzyme, and kinetic constants were unaffected in the labeled PNPs. The study suggests that mass-constrained femtosecond motions at the catalytic site of PNP can improve transition state barrier crossing by more frequent sampling of essential catalytic site contacts. </p>