Mechanistic Studies on the Aminopeptidase from Aeromonas proteolytica: A Two-Metal Ion Mechanism for Peptide Hydrolysis

Abstract

The aminopeptidase from Aeromonas proteolytica (AAP) is uncompetitively inhibited by fluoride ion at pH 8.0 with an inhibition constant (K_i) of 30 mM. Thus, fluoride inactivates AAP only after substrate binding, and only a single fluoride ion binds to AAP. On the other hand, chloride ion does not inhibit AAP up to concentrations of 2 M at pH 8.0. The pH dependence of fluoride inhibition of AAP was measured over the pH range 6.0−9.5. Between pH values of 6.0 and 9.0, fluoride ion acts as a pure uncompetitive inhibitor of AAP, and the K_i increases from 1.2 to 370 mM. From a plot of pK_i vs pH, a pK_a value of 7.0 ± 0.3 was extracted which corresponds to a single deprotonation process. At pH values higher than 9.0, the fluoride inhibition pattern changes to competitive. This change in inhibition pattern was attributed to a change in ionic strength or perhaps pH of the solution since fluoride ion was also found to become a competitive inhibitor of AAP at pH 8.0 in the presence of 2 M NaCl. These data, taken together with previous kinetic studies of mono- and dinuclear hydrolases with fluoride ion, suggest that a Zn(II)-bound water/hydroxide exists at the dimetal active site of AAP with a pK_a of 7.0 and that this water/hydroxide acts as the active site nucleophile. The hydrolysis of l-leucine-p-nitroanilide was measured spectrophotometrically in triplicate between 25 and 85 °C at eight substrate concentrations ranging from 5 to 800 μM. From these data, K_m values were derived at each temperature studied and were found to increase exponentially with increasing temperature. Moreover, the calculated V_max values were also found to increase over this temperature range, mimicking the K_m values. An Arrhenius plot was constructed from k_cat values and was found to be linear over the temperature range 25−85 °C, indicating that the rate-limiting step in AAP peptide hydrolysis is product formation and does not change as a function of temperature. From the slope of the line, the activation energy (E_a) was calculated to be 36.5 kJ/mol. The enthalpy and entropy of activation at 25 °C calculated over the temperature range 298−358 K were found to be 34.0 kJ/mol and −94.2 J/(mol·K), respectively. The free energy of activation at 25 °C was found to be 62.1 kJ/mol. Combination of the available X-ray crystallographic data with the present kinetic and thermodynamic results, as well as the previously reported kinetic and spectroscopic data, has allowed a detailed catalytic mechanism for AAP to be proposed.