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JBC, Vol. 251, Issue 10, 2922-2928, May, 1976
L. A. Bentle, R. E. Snoke and H. A. Lardy
When rat liver cytosolic P-enolpyruvate carboxykinase is purified, its
activity is no longer enhanced by incubation with 30 muM Fe2+. Ferrous ion
stimulation of the purified enzyme is restored by the addition of rat liver
cytosol. The agent responsible is a cytosolic protein, named P-enolpyruvate
carboxykinase ferroactivator, that was readily separated from the enzyme
during purification of the latter. A quantitative assay for P-enolpyruvate
carboxykinase ferroactivator is described. Subcellular fractionation of
livers from fasted rats shows that 98% of the combined mitochondrial and
cytosolic P-enolpyruvate carboxykinase ferroactivator activity resides in
the cytosol. Fasting does not produce significant change in this cytosolic
activity when compared to that of fed animals. Examination of various
tissue homogenates shows that the ferroactivator is found in liver, kidney,
erythrocytes, adipose tissue, and brain. No activity was detected in blood
serum or skeletal muscle. The ability to enhance the activity of purified
rat liver cytosolic P-enolpyruvate carboxykinase in the presence of Fe2+ is
not species specific. P-enolpyruvate carboxykinase ferroactivator may have
an important function in regulating enzyme activity in vivo.
A protein factor required for activation of phosphoenolpyruvate carboxykinase by ferrous ions
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