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J. Biol. Chem., Vol. 259, Issue 12, 7590-7596, 06, 1984
GS Kopf and VD Vacquier
Abalone sperm adenylate cyclase activity is particulate in nature and
displays a high Mg2+-supported activity (Mg2+/Mn2+ = 0.8) as compared to
other sperm adenylate cyclases. Approximately 90% of the enzyme activity in
crude homogenates is inhibited by EGTA in a concentration- dependent manner
which is overcome by added micromolar free Ca2+. The EGTA-inhibited
Ca2+-stimulated enzyme activity is also inhibited by phenothiazines. Added
calmodulin, however, has no effect on enzyme activity prepared from crude
homogenates. Preparation of a twice EGTA- extracted 48,000 X g pellet
fraction yields a particulate enzyme activity that can be stimulated 10-65%
by added calmodulin in the presence of micromolar free Ca2+. Detergent
extraction (1% Lubrol PX) of the EGTA-washed 48,000 X g pellet solubilizes
2-5% of the total particulate adenylate cyclase activity, and this
solubilized enzyme is activated up to 125% by calmodulin. The ability of
the different enzyme preparations to be stimulated by calmodulin is
inversely proportional to the endogenous calmodulin concentration.
Calmodulin stimulation of the Lubrol PX-solubilized enzyme is specific to
this Ca2+-binding protein and is mediated as an effect on the velocity of
the enzyme. This stimulation is completely Ca2+ dependent and is fully
reversible. These data suggest that the control of sperm cAMP synthesis by
changes in Ca2+ conductance may be mediated via this Ca2+-binding protein.
Characterization of a calmodulin-stimulated adenylate cyclase from abalone spermatozoa
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