Response
regulator signaling proteins and phosphatases of the haloacid
dehalogenase (HAD) superfamily share strikingly similar folds, active
site geometries, and reaction chemistry. Proteins from both families
catalyze the transfer of a phosphoryl group from a substrate to one
of their own aspartyl residues, and subsequent hydrolysis of the phosphoprotein.
Notable differences include an additional Asp that functions as an
acid/base catalyst and an active site well-structured prior to phosphorylation
in HAD phosphatases. Both features contribute to reactions substantially
faster than those for response regulators. To investigate mechanisms
underlying the functional differences between response regulators
and HAD phosphatases, we characterized five double mutants of the
response regulator CheY designed to mimic HAD phosphatases. Each mutant
contained the extra Asp paired with a phosphatase-inspired substitution
to potentially position the Asp properly. Only CheY DR (Arg as the
anchor) exhibited enhanced rates of both autophosphorylation with
phosphoramidate and autodephosphorylation compared to those of wild-type
CheY. Crystal structures of CheY DR complexed with MoO<sub>4</sub><sup>2–</sup> or WO<sub>4</sub><sup>2–</sup> revealed
active site hydrogen bonding networks similar to
those in HAD·substrate complexes, with the extra Asp positioned
for direct interaction
with the leaving group (phosphorylation) or nucleophile (dephosphorylation).
However, CheY DR reaction kinetics did not exhibit the pH sensitivities
expected for acid/base catalysis. Biochemical analysis indicated CheY
DR had an enhanced propensity to adopt the active conformation without
phosphorylation, but a crystal structure revealed unphosphorylated
CheY DR was not locked in the active conformation. Thus, the enhanced
reactivity of CheY DR reflected partial acquisition of catalytic and
structural features of HAD phosphatases
