Abstract:
To elucidate the functional role of Arg82 and Arg86 in the enzyme activity of binase, the extracellular ribonuclease of Bacillus intermedias, we used site-directed mutagenesis. On cleavage of various substrates the catalytic activity of binase mutant Arg86Ala is 2.7 x 103-7.7 X 103 times less than that of the native enzyme. The decrease in activity is determined preferentially by the decrease in the molecular rate constant k(cat) with a relatively small change of enzyme-substrate affinity, characterized by K(m). This is the expected result if Arg86 acts to lower the energy of a transition state of the reaction. The replacement of Arg82 by Ala causes a 519-fold activity decrease, depending on the substrate. We propose that this residue does not have a direct catalytic function in the molecular mechanism of the nase action and that the activity decrease of binase on the replacement of Arg82 by alanine is mediated by the effect of Arg82 on the pK of catalytic residues.