Influence of Estradiol-17beta on Progesterone and Estrogen Receptor mRNA Expression in Porcine Follicular Granulosa Cells during Short-Term, In Vitro Real-Time Cell Proliferation

Author:

Ciesiółka Sylwia1,Budna Joanna1,Jopek Karol1,Bryja Artur2,Kranc Wiesława2,Chachuła Adrian1,Borys Sylwia2,Dyszkiewicz Konwińska Marta3,Ziółkowska Agnieszka14,Antosik Paweł5,Bukowska Dorota5,Brüssow Klaus P.5,Bruska Małgorzata2,Nowicki Michał1,Zabel Maciej16ORCID,Kempisty Bartosz12ORCID

Affiliation:

1. Department of Histology and Embryology, Poznań University of Medical Sciences, 6 Święcickiego St., 60-781 Poznań, Poland

2. Department of Anatomy, Poznań University of Medical Sciences, 6 Święcickiego St., 60-781 Poznań, Poland

3. Department of Biomaterials and Experimental Dentistry, Poznań University of Medical Sciences, 70 Bukowska St., 60-812 Poznań, Poland

4. Department of Anatomy and Histology, Faculty of Medicine and Health Sciences, University of Zielona Gora, ul. Zyty 28, 65-046 Zielona Gora, Poland

5. Institute of Veterinary and Animal Science, Poznań University of Life Sciences, 52 Wojska Polskiego St., 60-628 Poznań, Poland

6. Department of Histology and Embryology, Wroclaw Medical University, 6a Chalubinskiego St., 50-368 Wroclaw, Poland

Abstract

Progesterone (P4) and estradiol (E2) play a significant role in mammalian reproduction. Our study demonstrated that separated porcine cumulus cells (CCs) and/or granulosa cells (GCs) might proliferate in vitro during short-term, real-time primary culture. The GCs were analyzed according to gene expression of the progesterone receptor (nuclear form) (pgr), progesterone receptor membrane component 1 (pgrmc1), and estrogen-related receptor beta 3 (esrrb3) in relation to two housekeeping genes: actb and pbgd. GCs were cultivated in medium with the E2. Both pgr/actb and pgr/pbgd revealed higher expression between 24 and 168 h of IVC of prolonged E2 treatment and at 48 h of IVC after acute E2 administration. The pgrmc1/actb and pgrmc1/pbgd displayed increased expression after prolonged E2 treatment between 24 and 120 h of IVC. The highest level of esrrb3/actb at 120 and 144 h, as well as esrrb3/pbgd at 120 h, in untreated controls as compared to the hormone-stimulated group, was observed. We suggest that E2 significantly influences the upregulation of pgr, pgrmc1, and esrrb3 expression in porcine GCs during real-time cell proliferation. Since esrrb3 expression is stimulated by E2 in both an acute and prolonged manner, estradiol may be recognized as a potential estrogen receptor agonist in GCs.

Funder

Polish National Centre of Science

Publisher

Hindawi Limited

Subject

General Immunology and Microbiology,General Biochemistry, Genetics and Molecular Biology,General Medicine

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