Reverse transphosphorylation by ribonuclease A needs an intact p sub(2)-binding site: Point mutations at Lys-7 and Arg-10 alter the catalytic properties of the enzyme

Bovine pancreatic ribonuclease A interacts with RNA along multiple binding subsites that essentially recognize the negatively charged phosphates of the substrate. This work gives additional strong support to the existence of the postulated phosphate-binding subsite p sub(2) and confirms the central role of Lys-7 and Arg-10 in establishing an electrostatic interaction with a phosphate group of the substrate. The effects of charge elimination by Lys-7 arrow right Gln (K7Q) and/or Arg-10 arrow right Gln (R10Q) substitutions in catalytic and ligand-binding properties of ribonuclease A have been studied. The values of K sub(m) for cytidine 2',3'-cyclic phosphate and cytidylyl-3',5'-adenosine are not altered but are significantly increased for poly(C). In all cases, k sub(cat) values are lower. Synthetic activity, i.e. the reversion of the transphosphorylation reaction, is reduced for K7Q and R10Q mutants and is practically abolished in the double mutant. Finally, the extent of the reaction of the mutants with 6-chloropurine-9- beta -D-ribofuranosyl 5'-monophosphate indicates that the phosphate ionic interaction in p sub(2) is weakened. Thus, p sub(2) modification alters both the catalytic efficiency and the extent of the processes in which an interaction of the phosphate group of the substrate or ligand with the p sub(2)-binding subsite is involved.