EFFECT OF MUTAGENESIS AT EACH OF 5 HISTIDINE-RESIDUES ON ENZYMATIC-ACTIVITY AND STABILITY OF RIBONUCLEASE-H FROM ESCHERICHIA-COLI

To examine the role of histidine residues in ribonuclease H from Escherichia coli, kinetic parameters for the enzymatic activity and conformational stabilities against guanidine hydrochloride denaturation of mutant enzymes, in which each of the five histidine residues was replaced with alanine, were determined and compared with the wild-type enzyme. The mutation of His83 resulted in a marked increase in K(m) along with an increase in k(cat). The mutation of His114 caused a large reduction in both the free energy of unfolding in water, DELTA-G(H2O), and the mid-point of the unfolding curve, [D]1/2. These results indicate that His83, which is one of the four well-exposed histidine residues in the crystal structure, is located close to a substrate-binding site, and His114, which is buried inside the protein molecule, contributes to the conformational stability, probably through the formation of a hydrogen bond with a main-chain carbonyl group. None of the histidine residues is required for activity.