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Transcriptional Down-Regulation of Human Gonadotropin-Releasing Hormone (GnRH) Receptor Gene by GnRH: Role of Protein Kinase C and Activating Protein 11
Clinical applications of GnRH agonists (GnRHa) are based primarily on the decrease in gonadotropin release after down-regulation of the GnRH receptor (GnRHR) by continuous GnRHa administration. However, the molecular mechanisms underlying the transcriptional regulation of the human GnRHR gene after...
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| Published in: | Endocrinology (Philadelphia) 2000-10, Vol.141 (10), p.3611-3622 |
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| Main Authors: | , , , , |
| Format: | Article |
| Language: | English |
| Online Access: | Get full text |
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| Summary: | Clinical applications of GnRH agonists (GnRHa) are based
primarily on the decrease in gonadotropin release after
down-regulation of the GnRH receptor (GnRHR) by continuous GnRHa
administration. However, the molecular mechanisms underlying the
transcriptional regulation of the human GnRHR gene after prolonged GnRH
treatment remain poorly understood. In the present study GnRHa-mediated
regulation of human GnRHR gene transcription was studied by transiently
transfecting the mouse gonadotrope-derived (αT3–1) cells with a
2297-bp human GnRHR promoter-luciferase construct (p2300-LucF). A
dose- and time-dependent decrease in human GnRHR promoter activity
was observed after GnRHa treatment. An average 71% decrease in
promoter activity was observed after 24-h treatment with 0.1μ
m GnRHa, which was blocked by cotreatment of the
GnRH antagonist, antide. This effect was mimicked by phorbol
12-myristate 13-acetate (TPA) administration. In addition, the
GnRHa- and TPA-mediated decrease in the human GnRHR promoter
activity was reversed by a specific protein kinase C (PKC) inhibitor,
GF109203X, or depletion of PKC by TPA pretreatment. These findings
indicate that the activation of the PKC pathway is important in
regulating the human GnRHR gene expression.
By progressive 5′-deletion studies, we have identified a 248-bp DNA
fragment (−1018 to −771, relative to the translation start site) at
the 5′-flanking region of the human GnRHR gene that is responsible for
the GnRHa-mediated down-regulation of human GnRHR promoter activity.
Analysis of this sequence reveals the existence of two putative
activating protein-1 (AP-1) sites with 87% homology to the
consensus sequence
(5′-TGAG/CTC/AA-3′),
located at −1000 to −994 (5′-TTAGACA-3′, in complementary
orientation) and −943 to −937 (5′-TGAATAA-3′). Using competitive
gel mobility shift assays, AP-1 binding was observed within this 248-bp
region. Site-directed mutation of the putative AP-1-binding site
located at −1000 to −994 abolished the GnRHa-induced inhibition.
Further competitive GMSA and supershift experiments confirmed the
identity of AP-1 binding in this region. By the use of Western blot
analysis, a significant increase in c-Jun (100%; P< 0.05) and c-Fos (50%; P < 0.05) protein levels
was observed after GnRHa treatment in αT3–1 cells. In addition, our
data suggested that a change in AP-1 composition, particularly c-Fos,
was important in mediating GnRHa-induced inhibition of human GnRHR gene
expression.
We conclude that acti |
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| ISSN: | 0013-7227 1945-7170 |
| DOI: | 10.1210/endo.141.10.7730 |