Expression of 11β-hydroxysteroid dehydrogenase, glucocorticoid receptor, and mineralocorticoid receptor genes in rat ovary

A new concept in reproductive endocrinology is that the status of the ovary as a glucocorticoid target organ alters with follicular development. Evidence for a physiological role of glucocorticoids in the regulation of ovarian folliculogenesis has been strengthened by the discovery that 11 beta -hyd...

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Veröffentlicht in:Biology of reproduction 1999-02, Vol.60 (2), p.330-335
Hauptverfasser: TETSUKA, M, MILNE, M, SIMPSON, G. E, HILLIER, S. G
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container_title Biology of reproduction
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creator TETSUKA, M
MILNE, M
SIMPSON, G. E
HILLIER, S. G
description A new concept in reproductive endocrinology is that the status of the ovary as a glucocorticoid target organ alters with follicular development. Evidence for a physiological role of glucocorticoids in the regulation of ovarian folliculogenesis has been strengthened by the discovery that 11 beta -hydroxysteroid dehydrogenase (11 beta HSD) mRNA expression in human granulosa cells is developmentally regulated. In this study, we quantified the pattern of expression and investigated the cellular location of 11 beta HSD type 1 (11 beta HSD1), 11 beta HSD type 2 (11 beta HSD2), glucocorticoid receptor (GR), and mineralocorticoid receptor (MR) mRNAs during follicular maturation in rat ovary. Immature female rats received treatment with eCG to induce preovulatory follicular development or eCG followed by hCG to induce luteinization. 11 beta HSD1, 11 beta HSD2, GR, and MR mRNAs were all detectable by ribonuclease protection assay in ovarian total RNA. Treatment with eCG alone caused an similar to 8-fold increase in the ovarian level of 11 beta HSD1 mRNA, which rose to similar to 30-fold after additional treatment with hCG. Equine CG alone did not measurably affect the ovarian 11 beta HSD2 mRNA level, but additional treatment with hCG reduced it to 34% of the control level. Expression of GR mRNA was unchanged by any gonadotropin treatment, while MR mRNA was down-regulated. A similar pattern of 11 beta HSD1, 11 beta HSD2, GR, and MR mRNA expression was observed in isolated granulosa cells. These results provide direct experimental evidence that 11 beta HSD genes are gonadotropically regulated in the rat ovary, including granulosa cells, and are consistent with a shift in glucocorticoid metabolism from inactivation (due to oxidation by 11 beta HSD2) to activation (reduction by 11 beta HSD1) during hCG-induced granulosa cell luteinization.
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Immature female rats received treatment with eCG to induce preovulatory follicular development or eCG followed by hCG to induce luteinization. 11 beta HSD1, 11 beta HSD2, GR, and MR mRNAs were all detectable by ribonuclease protection assay in ovarian total RNA. Treatment with eCG alone caused an similar to 8-fold increase in the ovarian level of 11 beta HSD1 mRNA, which rose to similar to 30-fold after additional treatment with hCG. Equine CG alone did not measurably affect the ovarian 11 beta HSD2 mRNA level, but additional treatment with hCG reduced it to 34% of the control level. Expression of GR mRNA was unchanged by any gonadotropin treatment, while MR mRNA was down-regulated. A similar pattern of 11 beta HSD1, 11 beta HSD2, GR, and MR mRNA expression was observed in isolated granulosa cells. 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source Oxford University Press Journals All Titles (1996-Current); EZB-FREE-00999 freely available EZB journals
subjects Biological and medical sciences
Fundamental and applied biological sciences. Psychology
Hormone metabolism and regulation
Mammalian female genital system
Vertebrates: reproduction
title Expression of 11β-hydroxysteroid dehydrogenase, glucocorticoid receptor, and mineralocorticoid receptor genes in rat ovary
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