In vitro decidualization of human endometrial stromal cells

doi:10.1016/0960-0760(92)90137-8

The Journal of Steroid Biochemistry and Molecular Biology

Volume 42, Issues 3–4, May 1992, Pages 337-344

https://doi.org/10.1016/0960-0760(92)90137-8 Get rights and content

Abstract

Stromal cells isolated from proliferative human endometrium undergo morphologic and biochemical changes when exposed to a mixture of ovarian hormones, acquiring characteristics of decidual cells. In addition to the previously reported progestin-induced secretion of prolactin (PRL) by explants of human proliferative endometrium, and of PRL and laminin by stromal cells in culture, “in vitro” induction of several other decidual cell products was demonstrated in the present study, using cultures of stromal cells isolated from proliferative endometrium.

Incubation of stromal cells with a mixture of estradiol, medroxyprogesterone acetate and relaxin, at a concentration reported to yield maximal stimulation of PRL production, resulted in changes from elongated to rounder cells, approx. 90% of which showed immunostaining for PRL under these conditions. Immunocytochemical procedures were carried out on cytospins of decidual cells isolated from decidual tissue adherent to fetal membranes collected at delivery (positive controls), and on stromal cells cultured in Lab-Tek chamber-slides, in the absence (negative controls) or in the presence of added hormones. Antibodies to 24K (a heat-shock protein also named HRP27), desmin (present in intermediate filaments), p29 (a protein associated with the estrogen receptor), and PP12 (an insulin growth factor-1 binding protein), did not react with stromal cells isolated from proliferative endometrium but showed immunostaining of the rounder cells obtained after hormonal treatment when tested with the peroxidase-labeled second antibody complex. In another series of similar experiments, in which the same decidualization end-points were emploted, changes in 24K, desmin and PP12 expression were obtained by adding to the insulin-containing medium PRL instead of the hormonal mixture, a finding suggesting sequential steps during the decidualization process.

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Cited by (127)

The fate of human SUSD2+ endometrial mesenchymal stem cells during decidualization
2022, Stem Cell Research
Regeneration of the endometrial stromal compartment in premenopausal women is likely maintained by the perivascular endometrial mesenchymal stem/stromal cells (eMSC) expressing sushi domain containing 2 (SUSD2). The fate of SUSD2+ eMSC during pregnancy and their role in decidualization is not fully known. The aim of our study was to determine the effect of progesterone on the stemness of the SUSD2+ eMSC isolated from non-pregnant uterine samples. Secondary objectives were to characterize the functional capacity including differentiation and clonogenicity assays of SUSD2+ eMSC isolated from decidua at full term and compare it to the capacity of those isolated from non-pregnant uterine samples. Progesterone treatment induced changes in the decidual gene expression profile in non-pregnant SUSD2+ eMSC. Data analysis of a publicly available single cell RNA-seq data set revealed differential expression of several mesenchymal and epithelial signature genes between the SUSD2+ eMSC and the decidual stromal cells, suggesting mesenchymal-to-epithelial transition occurs during decidualization. Histological analysis revealed a significantly lower abundance of SUSD2+ eMSC in 1^s^t trimester and full term samples compared to non-pregnant samples, p = 0.0296 and 0.005, respectively. The differentiation and the colony forming capacity did not differ significantly between the cells isolated from non-pregnant and pregnant uterine samples. Our results suggest that SUSD2+ eMSC undergo decidualization in vitro, while maintaining MSC plasma membrane phenotype. Human eMSC seem to play an important role in the course of endometrial decidualization and embryo implantation. Pregnancy reduced the abundance of SUSD2+ eMSC, however eMSC function remains intact.
Introduction: Endometrial function: facts, urban legends, and an eye to the future
2017, Fertility and Sterility
Citation Excerpt :
This transformation begins in the midsecretory phase of the menstrual cycle around uterine spiral arterioles, immediately after the plasma membrane transformation that occurs in the luminal epithelium that is mandatory for the acquisition of endometrial receptivity (3). Decidualization is driven by the postovulatory or endogenous rise in progesterone levels, increasing local cyclic adenosine monophosphate production (4–6), which stimulates synthesis of a complex network of intracellular and secreted proteins (7). Morphologically, this process is characterized by the transformation of elongated fibroblast-like stromal cells (ESCs) into enlarged polygonal/round cells shaped by a complex intracellular cytoskeleton rearrangement (8, 9).
The embryo alone, though very important, is not sufficient to explain successful or failed implantation. Human embryonic implantation is less efficient than in nonmenstruating species. The main difference lies in the decidual control of early implantation events and the subsequent course of pregnancy versus embryo control in nonmenstruating species. In this article, we introduce the facts behind the low efficiency of this crucial process, address urban legends routinely considered without high clinical quality evidence, and provide a vision of how the endometrial field will develop in the near future.
Spontaneous decidualization in pseudopregnant rats with vitamin e deficiency
2016, Biochemical and Biophysical Research Communications
Successful implantation of an embryo requires adequate depth of invasion in the endometrium, which depends upon decidualization. The aim of the present study was to elucidate why humans experience spontaneous decidualization and menstruation while most other mammals do not. We established a spontaneous decidualization model in pseudopregnant rats with vitamin E deficiency (VED) to investigate mechanisms associated with spontaneous decidualization. Vaginal smears were used to monitor bleeding while vitamin E levels were analyzed with a commercial vitamin E assay kit. Trypan blue staining was used to observe the implantation site at 5.5 days post-coitum (dpc). Uterine morphology, estradiol (E₂) and progesterone levels, and the anti-oxidation system were evaluated at 5.5, 7.5, and 9.5 dpc. The proportion of rats in the VED group exhibiting endometrial bleeding gradually increased (5.9%, 32.3%, and 50%) over three consecutive cycles of pseudopregnancy. Vitamin E levels in the VED group were markedly lower compared to the control group in both the plasma and uterus, while the level of vitamin E in the liver did not differ between the control and VED groups. Spontaneous decidualization in the VED group was validated by histological examination and immunohistochemistry. At 5.5 dpc, the mean serum E₂ level in the VED group was more than twice that of the control group. The mean total anti-oxidizing capability, catalase level, and glutathione peroxidase activity were significantly reduced in the decidualized portion of the VED group compared to controls, while the malondialdehyde level was also significantly higher in the decidualized portion of the VED group. We hypothesize that the E₂ surge at 5.5 dpc and increasing levels of reactive oxygen species are responsible for spontaneous decidualization in VED rats.
Cyclic processes in the uterine tubes, endometrium, myometrium, and cervix: pathways and perturbations
2023, Molecular Human Reproduction
Immune Tolerance of Embryo Implantation and Pregnancy: The Role of Human Decidual Stromal Cell- and Embryonic-Derived Extracellular Vesicles
2022, International Journal of Molecular Sciences
Energy deficiency caused by CTPS downregulation in decidua may contribute to pre-eclampsia by impairing decidualization
2021, Journal of Cellular Physiology

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^∗: Present address: Reproductive Medicine Unit, Department of Obstetrics and Gynecology, University of Bologna, Bologna, Italy.

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The Journal of Steroid Biochemistry and Molecular Biology

Abstract

References (26)

Endometrial morphology of women using a d-norgestrel-releasing intrauterine device

Fert. Steril.

Endometrium in term extrauterine pregnancy

Human Pathol.

Hormonal regulation of human endometrial stromal cells in culture: an in vitro model for decidualization

Fert. Steril.

An estrogen-related protein in normal and malignant endometrium

J. Steroid Biochem.

Immunochemical and biochemical relationship between human pregnancy associated secreted endometrial 1 and 2 globulins and the soluble placental proteins 12 and 14 (PP12 and PP14)

Placenta

Expression of desmin, laminin and fibronectin during in situ differentiation (decidualization) of rat uterine stromal cells

Differentiation

Characterization of p29, an estrogen receptor associated tumor marker

J. Steroid Biochem.

Characterization and biological relevance of a 29-kDa estrogen receptor-related protein

J. Steroid Biochem.

Dating the endometrial biopsy

Fert. Steril.

Mouse endometrial stromal cells produce basement-membrane components

Differentiation

Induction and maintenace of decidual changes with progesterone and estrogen

J. Clin. Endocr. Metab.

Cited by (127)

The fate of human SUSD2+ endometrial mesenchymal stem cells during decidualization

Introduction: Endometrial function: facts, urban legends, and an eye to the future

Spontaneous decidualization in pseudopregnant rats with vitamin e deficiency

Cyclic processes in the uterine tubes, endometrium, myometrium, and cervix: pathways and perturbations

Immune Tolerance of Embryo Implantation and Pregnancy: The Role of Human Decidual Stromal Cell- and Embryonic-Derived Extracellular Vesicles

Energy deficiency caused by CTPS downregulation in decidua may contribute to pre-eclampsia by impairing decidualization