Yassmin Medina-Laver scite author profile

The progesterone hormone regulates the human menstrual cycle, pregnancy, and parturition by its action via the different progesterone receptors and signaling pathways in the female reproductive tract. Progesterone actions can be exerted through classical and non-classical receptors, or even a combination of both. The former are nuclear receptors whose activation leads to transcriptional activity regulation and thus in turn leads to slower but long-lasting responses. The latter are composed of progesterone receptors membrane components (PGRMC) and membrane progestin receptors (mPRs). These receptors rapidly activate the appropriate intracellular signal transduction pathways, and they can subsequently initiate specific cell responses or even modulate genomic cell responses. This review covers our current knowledge on the mechanisms of action and the relevance of classical and non-classical progesterone receptors in female reproductive tissues ranging from the ovary and uterus to the cervix, and it exposes their crucial role in female infertility.

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Mercury impairs human primary endometrial stromal cell function

Palomar

González-Martín

Pérez-Debén

et al. 2022

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Heavy metal exposures could compromise endometrial cells and decidualization. Although studies assessed mercury toxicity in cell lines, limited data are available on the concentration of mercury that induces damage in hEnSC, which could alter endometrial function. This research aims to study effects of mercury exposure on cell viability and functional features of hEnSC. Primary hEnSC were isolated from 23 endometrial biopsies obtained from healthy egg donors. After in vitro mercury exposure or control treatment of hEnSC, cell viability was evaluated via tetrazolium salt metabolism and oxidative stress was assessed by 2′,7’-DCFDA assay. hEnSC were decidualized in vitro in the presence of mercury (0, 25, 50, 75, 250 and 350 nM). Decidualization was evaluated based on prolactin and IGFBP1 secretion and cytoskeletal rearrangement (F-actin staining). Cell proliferation and apoptosis were evaluated by Ki67 immunostaining and TUNEL assay. Mercury doses of 250 nM (p = 0.028) and 500 nM (p = 0.026) increased ROS production in hEnSC after 24 h. Cell viability significantly decreased after 48 h and 72 h (p = 0.032 and p = 0.016, respectively) of mercury exposure at 500 nM. After in vitro decidualization and mercury treatment, decidual hEnSC showed a dose-dependent decrease in prolactin and IGFBP1 secretion, particularly at 350 nM (p = 0.016). Cell proliferation was decreased in hEnSC treated with 350 nM mercury (p < 0.001); an increase in apoptosis followed a dose-dependent trend in non-decidual and decidual hEnSC. These findings support that mercury-induced damage could be due to an increase in ROS production.

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Endometrial Cells Acutely Exposed to Phthalates In Vitro Do Not Phenocopy Endometriosis

González-Martín

Palomar

Medina-Laver

et al. 2022

IJMS

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Environmental factors that have been linked to an increased endometriosis risk include exposure to di-(2-ethylhexyl)-phthalate (DEHP), an endocrine disruptor. This study aims to investigate whether DEHP in vitro exposure in primary endometrial stromal cells (EnSC), primary endometrial epithelial cells (EnEC), and the human endometrial adenocarcinoma cell line Ishikawa properly mimics alterations described in the eutopic endometrium of women with endometriosis. Primary EnSC and EnEC, isolated from six fertile egg donors, and Ishikawa cells were exposed to DEHP (0.1, 1, and 10 µM) and were assessed for viability, endometriosis markers (IL-6, VEGF-A, HOXA10, EZH2, and LSD1), steroid receptor gene expressions (ER-1, ER-2, PR-T, PR-B, and PGRMC1), and invasive capacity. Viability after 72 h of DEHP exposure was not significantly affected. None of the endometriosis markers studied were altered after acute DEHP exposure, nor was the expression of steroid receptors. The invasive capacity of EnSC was significantly increased after 10 µM of DEHP exposure. In conclusion, acute DEHP exposure in primary endometrial cells does not fully phenocopy the changes in the viability, expression of markers, or steroidal receptors described in endometriosis. However, the significant increase in EnSC invasiveness observed after DEHP exposure could be a link between DEHP exposure and increased endometriosis likelihood.

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Antioxidant Supplementation Alleviates Mercury-Induced Cytotoxicity and Restores the Implantation-Related Functions of Primary Human Endometrial Cells

Palomar

Quiñonero

Medina-Laver

et al. 2023

IJMS

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Mercury (Hg) cytotoxicity, which is largely mediated through oxidative stress (OS), can be relieved with antioxidants. Thus, we aimed to study the effects of Hg alone or in combination with 5 nM N-Acetyl-L-cysteine (NAC) on the primary endometrial cells’ viability and function. Primary human endometrial epithelial cells (hEnEC) and stromal cells (hEnSC) were isolated from 44 endometrial biopsies obtained from healthy donors. The viability of treated endometrial and JEG-3 trophoblast cells was evaluated via tetrazolium salt metabolism. Cell death and DNA integrity were quantified following annexin V and TUNEL staining, while the reactive oxygen species (ROS) levels were quantified following DCFDA staining. Decidualization was assessed through secreted prolactin and the insulin-like growth factor-binding protein 1 (IGFBP1) in cultured media. JEG-3 spheroids were co-cultured with the hEnEC and decidual hEnSC to assess trophoblast adhesion and outgrowth on the decidual stroma, respectively. Hg compromised cell viability and amplified ROS production in trophoblast and endometrial cells and exacerbated cell death and DNA damage in trophoblast cells, impairing trophoblast adhesion and outgrowth. NAC supplementation significantly restored cell viability, trophoblast adhesion, and outgrowth. As these effects were accompanied by the significant decline in ROS production, our findings originally describe how implantation-related endometrial cell functions are restored in Hg-treated primary human endometrial co-cultures by antioxidant supplementation.

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