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JBC, Vol. 250, Issue 19, 7795-7801, Oct, 1975
Comparison of adenosine 3':5'-monophosphate-dependent protein kinases from rabbit skeletal and bovine heart muscle
F. Hofmann, J. A. Beavo, P. J. Bechtel and E. G. Krebs
Homogeneous preparations of adenosine 3':5'-monophosphate (cyclic
AMP)-dependent protein kinase from rabbit skeletal (Peak I) and bovine
heart muscle have been compared. Each enzyme has an S20,w value of 7.0.
Each enzyme binds 2 mol of cyclic AMP per mol of enzyme and is dissociated
in the presence of saturating concentrations of cyclic AMP into a demeric
regulatory subunit-cyclic AMP complex and two catalytic subunits. The
isolated subunits recombine, resulting in the formation of the original
holoenzyme in each case. Several differences between the two enzymes were
found. Different salt concentrations are necessary for elution of the
respective enzyme from DEAE-cellulose. Their regulatory subunits differ
with respect to their sedimentation constants and mobility on sodium
dodecyl sulfate gel electrophoresis. The regulatory subunit of the heart
enzyme is rapidly phosphorylated by MgATP but this does not occur with the
skeletal muscle enzyme. MgATP is bound with high affinity only to the
skeletal muscle enzyme. The enzymes have different apparent dissociation
constants and Hill coefficients for cyclic AMP binding. With the skeletal
muscle enzyme MgATP increases the dissociation constants for cyclic AMP
about 10-fold and decreases the Hill coefficient, while with the heart
enzyme phosphorylation decreases the cissociation constant for cyclic AMP
5- to 6-fold and increases the Hill coefficient. Different concentrations
of cyclic AMP are required to dissociate the skeletal and heart muscle
enzymes. The presence of MgATP increases the concentration of cyclic AMP
required to dissociate the skeletal muscle enzyme but decreases the
concentration necessary to dissociate the heart enzyme.

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Copyright © 1975 by the American Society for Biochemistry and Molecular Biology.
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