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Endocrinology, doi:10.1210/en.2004-0092
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Endocrinology Vol. 145, No. 8 3594-3602
Copyright © 2004 by The Endocrine Society

Regulation of Gonadotropin-Releasing Hormone Receptors by Protein Kinase C: Inside Out Signalling and Evidence for Multiple Active Conformations

Christopher J. Caunt, James N. Hislop, Eamonn Kelly, Anne-Lise Matharu, Lisa D. Green, Kathleen R. Sedgley, Ann R. Finch and Craig A. McArdle

Laboratories for Integrative Neuroscience and Endocrinology (C.J.C., L.D.G., K.R.S., A.R.F., C.A.M.), and Department of Pharmacology (E.K., A.-L.M.), University of Bristol, Bristol BS1 3NY, United Kingdom; and University of California, San Francisco (J.N.H.), San Francisco, California 94143-2140

Address all correspondence and requests for reprints to: Craig A. McArdle, Henry Wellcome Laboratories for Integrative Neuroscience and Endocrinology, University of Bristol, Bristol BS1 3NY, United Kingdom. E-mail: craig.mcardle{at}bris.ac.uk.

Desensitization and internalization of G protein-coupled receptors can be mediated by phosphorylation within the C-terminal tail, facilitating ß-arrestin binding and targeting the receptor for internalization. Type II GnRH receptors (GnRH-Rs) show such regulation, but type I GnRH-Rs lack C-tails and are not rapidly desensitized or internalized. Here we show contrasting susceptibility of type I (human and sheep) and II (Xenopus) GnRH-Rs to regulation by protein kinase C (PKC). When human (h) or Xenopus (X) GnRH-Rs were expressed using recombinant adenovirus, PKC activation increased radioligand binding to XGnRH-Rs but not to hGnRH-Rs. A dominant-negative dynamin mutant (K44A) inhibited internalization of XGnRH-Rs (but not hGnRH-Rs) without influencing PKC regulation of XGnRH-R binding. PKC activation increased the affinity of XGnRH-Rs for the type II GnRH ligand and increased effects of low concentrations of GnRH-II on the [Ca2+]i but had no effect on type I ligand binding to hGnRH-Rs, sGnRH-Rs or XGnRH-Rs, or to chimeric receptors with the XGnRH-R C-tail added to a type I receptor. Binding of type II ligand to human or sheep receptors was also unaffected but was increased in the chimeras. Mutation of both PKC-phosphorylation consensus sites in the XGnRH-R tail did not prevent the PKC-mediated increases in binding or alter agonist-induced translocation of ß-arrestin2/green fluorescent protein or inhibition of inositol phosphate accumulation by ß-arrestin2/green fluorescent protein. Thus, it appears that there are two distinct active conformations of XGnRH-Rs (differing in affinity for type I and II ligands) and that these cells exhibit a novel form of inside-out signaling in which PKC feeds back to influence receptor affinity.




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