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J. Biol. Chem., Vol. 261, Issue 4, 1724-1729, Feb, 1986
WJ Harvey and R Blostein
In situ proteolysis of Na,K-ATPase was studied using inside-out red cell
membrane vesicles. Proteolysis of the enzyme in its "E1" conformation with
either trypsin or chymotrypsin inactivated cation translocation more than
ATP hydrolysis. This was evident both in the absence of intravesicular
alkali cations when Na-ATPase was compared to ATP-dependent 22Na+ influx,
and in the presence of K+ when Na+/K+ exchange was compared to (Na+ +
K+)-activated ATPase. This differential loss in pump versus hydrolysis was
observed also when the activities of only intact, non-leaky vesicles were
compared and therefore reflects intramolecular uncoupling rather than
nonspecific leakage. Although oligomycin and thimerosal, like trypsin and
chymotrypsin, inhibit the enzyme's conformational step(s), neither effect
uncoupling. It is concluded that specific cleavage(s) of Na,K-ATPase, at
least as it exists in situ, alters the reaction sequence with respect to
the normal ordered mechanism. Accordingly, cytoplasmic Na+ and
extracellular K+ bind to the enzyme, stimulate phosphorylation (ATP +
E1----E1P + ADP) and dephosphorylation (E2P----E2 + Pi), respectively, but
each is then released to the same side from which it had bound; presumably
release occurs prior to the conformational transitions of E1P to E2P and E2
to E1. This conclusion is supported by experiments showing that, ar
micromolar ATP concentration, the hydrolytic activity (Na-ATPase) of the
trypsinized but not the unmodified enzyme is stimulated by K+, consistent
with earlier experiments (Hegyvary, C., and Post, R. L. (1971) J. Biol.
Chem. 246, 5234-5240) showing that the K X E2 to K X E1 transition is
slower than the E2 to E1 transition.
Uncoupling the red cell sodium pump by proteolysis
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