The AF-1 Activation Function of Estrogen Receptor α Is Necessary and Sufficient for Uterine Epithelial Cell Proliferation In Vivo

Author:

Abot Anne1,Fontaine Coralie1,Raymond-Letron Isabelle2,Flouriot Gilles3,Adlanmerini Marine1,Buscato Melissa1,Otto Christiane4,Bergès Hortense1,Laurell Henrik1,Gourdy Pierre1,Lenfant Françoise1,Arnal Jean-François1

Affiliation:

1. Institut National Scientifique de la Santé et de la Recherche Médicale (INSERM) U1048 (A.A., C.F., M.A., M.B., H.B., H.L., P.G., F.L., J.-F.A.), Institut des Maladies Métaboliques et Cardiovasculaires, Université Paul Sabatier, BP 84225, 31 432 Toulouse cedex 04, France

2. Université de Toulouse (I.R.-L.), Institut National Polytechnique, Ecole Nationale Vétérinaire de Toulouse, F-31076 Toulouse, France

3. Université de Rennes I (G.F.), Centre National de la Recherche Scientifique, Unité Mixte de Recherche 6026 Équipe “Récepteur des oestrogènes et destinée cellulaire”, Campus de Beaulieu, 35042 Rennes Cedex, France

4. Therapeutic Research Group Oncology & Gynecological Therapy (C.O.), Bayer Pharma AG, 13342 Berlin, Germany

Abstract

Abstract Estrogen receptor-α (ERα) regulates gene transcription through the 2 activation functions (AFs) AF-1 and AF-2. The crucial role of ERαAF-2 was previously demonstrated for endometrial proliferative action of 17β-estradiol (E2). Here, we investigated the role of ERαAF-1 in the regulation of gene transcription and cell proliferation in the uterus. We show that acute treatment with E2 or tamoxifen, which selectively activates ERαAF-1, similarly regulate the expression of a uterine set of estrogen-dependent genes as well as epithelial cell proliferation in the uterus of wild-type mice. These effects were abrogated in mice lacking ERαAF-1 (ERαAF-10). Four weeks of E2 treatment led to uterine hypertrophy and sustained luminal epithelial and stromal cell proliferation in wild-type mice, but not in ERαAF-10 mice. However, ERαAF-10 mice still presented a moderate uterine hypertrophy essentially due to a stromal edema, potentially due to the persistence of Vegf-a induction. Epithelial apoptosis is largely decreased in these ERαAF-10 uteri, and response to progesterone is also altered. Finally, E2-induced proliferation of an ERα-positive epithelial cancer cell line was also inhibited by overexpression of an inducible ERα isoform lacking AF-1. Altogether, these data highlight the crucial role of ERαAF-1 in the E2-induced proliferative response in vitro and in vivo. Because ERαAF-1 was previously reported to be dispensable for several E2 extrareproductive protective effects, an optimal ERα modulation could be obtained using molecules activating ERα with a minimal ERαAF-1 action.

Publisher

The Endocrine Society

Subject

Endocrinology

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