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José C Garrido-Gracia Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Ana Gordon Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Carmina Bellido Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Rafaela Aguilar Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Inmaculada Barranco Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Yolanda Millán Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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Juana Martín de las Mulas Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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José E Sánchez-Criado Departments of Cell Biology, Physiology and Immunology and
Comparative Pathology, University of Córdoba, Córdoba, Spain

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The specific role of each oestrogen receptor (ER) isoform (α and β ) and site (nucleus and plasma membrane) in LH release was determined in ovariectomized (OVX) rats injected over 6 days (days 15–20 after OVX) with a saturating dose (3 mg/day) of tamoxifen (TX), a selective ER modulator with nuclear ERα agonist actions in the absence of oestrogen. This pharmacological effect of TX was demonstrated by the fact that it was blocked by the selective ERα antagonist methyl-piperidinopyrazole. Over the past 3 days of the 6-day TX treatment, rats received either 25 μg/day oestradiol benzoate (EB), 1.5 mg/day selective ERα agonist propylpyrazole triol (PPT) and the selective ERβ agonist diarylpropionitrile (DPN), or a single 3 mg injection of the antiprogestin onapristone (ZK299) administered on day 20. Blood samples were taken to determine basal and progesterone receptor (PR)-dependent LH-releasing hormone (LHRH)-stimulated LH secretion and to evaluate LHRH self-priming, the property of LHRH that increases gonadotrope responsiveness to itself. Blood LH concentration was determined by RIA and gonadotrope PR expression by immunohistochemistry. Results showed that i) EB and DPN potentiated the negative feedback of TX on basal LH release; ii) DPN reduced TX-induced PR expression; iii) EB and PPT blocked TX-elicited LHRH self-priming and iv) ZK299 reduced LHRH-stimulated LH secretion and blocked LHRH self-priming. These observations suggest that oestrogen action on LH secretion in the rat is exerted at the classic ERα pool and that this action might be modulated by both ERβ and membrane ERα through their effects on PR expression and action respectively.

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Ana Gordon Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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José C Garrido-Gracia Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Rafaela Aguilar Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Carmina Bellido Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Juan A García Velasco Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Yolanda Millan Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Manuel Tena-Sempere Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Juana Martín de las Mulas Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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José E Sánchez-Criado Cell Biology, Comparative Pathology, IVI Madrid, Departments of

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Hyperstimulation of ovarian function with human FSH (hFSH) attenuates the preovulatory surge of LH. These experiments aimed at investigating the mechanism of ovarian-mediated FSH suppression of the progesterone (P4) receptor (PR)-dependent LH surge in the rat. Four-day cycling rats were injected with hFSH, oestradiol benzoate (EB) or vehicle during the dioestrous phase. On pro-oestrus, their pituitaries were studied for PR mRNA and protein expression. Additionally, pro-oestrous pituitaries were incubated in the presence of oestradiol-17β (E2), and primed with P4 and LH-releasing hormone (LHRH), with or without the antiprogestin RU486. After 1 h of incubation, pituitaries were either challenged or not challenged with LHRH. Measured basal and LHRH-stimulated LH secretions and LHRH self-priming were compared with those exhibited by incubated pituitaries on day 4 from ovariectomized (OVX) rats in metoestrus (day 2) injected with hFSH and/or EB on days 2 and 3. The results showed that: i) hFSH lowered the spontaneous LH surge without affecting basal LH and E2 levels, gonadotroph PR-A/PR-B mRNA ratio or immunohistochemical protein expression; ii) incubated pro-oestrous pituitaries from hFSH-treated rats did not respond to P4 or LHRH, and lacked E2-augmenting and LHRH self-priming effects and iii) OVX reversed the inhibitory effects of hFSH on LH secretion. It is concluded that under the influence of hFSH, the ovaries produce a non-steroidal factor which suppresses all PR-dependent events of the LH surge elicited by E2. The action of such a factor seemed to be due to a blockade of gonadotroph PR action rather than to an inhibition of PR expression.

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