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Molecular Pharmacology, Vol 18, 362-369, Copyright © 1980 by the American Society for Pharmacology and Experimental Therapeutics
-Adrenergic Receptors by N-Ethylmaleimide in S49
Lymphoma Cells
1 Department of Pharmacology, Case Western Reserve University, School of Medicine, Cleveland, Ohio 44106
-Adrenergic agonists appear to induce a conformational change in 65% of the -adrenergic receptors in wild-type S49 lymphoma cell membranes as shown by the increased
sensitivity of a subpopulation of receptor to inactivation by the alkylating agent N-ethylmaleimide (NEM). This inactivation is conveniently monitored through the induction with NEM of a biphasic (-)-isoproterenol displacement curve of [125I]IHYP binding
to the receptors. In marked contrast, NEM alone or NEM plus a -adrenergic antagonist
has no effect on receptor binding. The final percentage (65%) of total receptor sites
inactivated with agonist plus NEM is not dependent on the concentration of NEM used
or on the time of exposure. Agonist plus NEM also causes inactivation of about 75% of
the receptors in the S49 lymphoma d clone, which has about 25% of the -adrenergic
receptor density of wild-type cells. However, agonist plus NEM treatment does not affect
receptor binding in unc and cyc- S49 cell membranes, in which the receptors are
functionally uncoupled from the adenylate cyclase complex. Further, agonists plus NEM
also cause inactivation of 45 to 60% of the -adrenergic receptors in turkey erythrocyte
membranes, but have no effect on solubilized receptors from the same cell. These findings
with variant S49 lines and turkey erythrocytes suggest that the ability of agonists to
produce a conformational change of -adrenergic receptors may be dependent on the
ability of these receptors to interact with the adenylate cyclase complex and specifically
to interact with the guanine nucleotide regulatory protein. The fact that only a given
fraction of the total receptor population can undergo a conformational change in the
investigated membranes and that the properties of the agonist/NEM-sensitive population
of receptors but not the insensitive population are similar to those of receptors which
activate adenylate cyclase suggests that, for structural or stoichiometric reasons, only
part of the receptor population can be coupled to the cyclase complex in the presence of
agonists. Thus agonist appears to induce a quantifiable, functional heterogeneity in an
apparently molecularly homogeneous receptor population.
Note:
ACKNOWLEDGMENTS
The skillful technical assistance of Paula L. Jacobs is greatly appreciated. We thank Dr. Henry Bourne for cultures of the d variant of
the S49 cell line.
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