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J. Biol. Chem., Vol. 262, Issue 14, 6489-6493, May, 1987
D Sugden and DC Klein
Rat pineal hydroxyindole-O-methyltransferase activity in crude homogenates
is reduced by treatment with disulfides. Cystamine (IC50 = 128 microM) and
selenocystamine (IC50 = 13 microM) are the most potent compounds tested.
Reduced cystamine (cysteamine) and diaminohexane are inactive.
N,N'-Diacetylcystamine, penicillamine disulfide, and glutathione disulfide
are less potent or inactive; but several peptides (oxytocin, vasopressin,
and arginine vasotocin) are active. Inactivation by cystamine is time- and
temperature-dependent and is accelerated at higher pH. Disulfide treatment
of intact pinealocytes also inactivates the enzyme. Addition of
dithiothreitol during the enzyme assay completely reactivates inactivated
enzyme formed by disulfide treatment of homogenates or intact cells. Rat
hydroxyindole-O- methyltransferase is also inactivated in the absence of
added disulfides and dissolved O2. This spontaneous inactivation is time-,
temperature-, and pH-dependent and can be completely prevented, but not
reversed, by dithiothreitol. In contrast to the inhibitory effects of
cystamine on the rat enzyme, cystamine does not alter bovine
hydroxyindole-O-methyltransferase and increases ovine hydroxyindole-O-
methyltransferase activity. The bovine and ovine enzymes do not become
inactive in the absence of added disulfides. Together these observations
indicate that rat pineal hydroxyindole-O-methyltransferase can be
inactivated by a protein thiol:disulfide exchange mechanism. This mechanism
may contribute to the physiological regulation of this enzyme in the rat
pineal gland but does not appear to be a common feature of pineal
hydroxyindole-O-methyltransferase regulation in all species.
Inactivation of rat pineal hydroxyindole-O-methyltransferase by disulfide-containing compounds
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