在蜕膜化过程中,子宫内膜基质细胞 miR-19b-3p 的释放减少,提示其在蜕膜-滋养层细胞相互作用中发挥作用。
Endometrial stromal cell miR-19b-3p release is reduced during decidualization implying a role in decidual-trophoblast cross-talk.
机构信息
Embryo Implantation Laboratory, Department of Obstetrics and Gynecology, The University of Melbourne, Parkville, VIC, Australia.
Gynecology Research Centre, The Royal Women's Hospital, Parkville, VIC, Australia.
出版信息
Front Endocrinol (Lausanne). 2023 Mar 16;14:1149786. doi: 10.3389/fendo.2023.1149786. eCollection 2023.
INTRODUCTION
A healthy pregnancy requires successful blastocyst implantation into an adequately prepared or 'receptive' endometrium. Decidualization of uterine endometrial stromal fibroblast cells (hESF) is critical for the establishment of a healthy pregnancy. microRNAs (miRs) are critical regulators of cellular function that can be released by a donor cell to influence the physiological state of recipient cells. We aimed to determine how decidualization affects hESF miR release and investigated the function of one decidualization regulated miR, miR-19b-3p, previously shown to be associated with recurrent pregnancy loss.
METHOD
miR release by hESF was determined by miR microarray on culture media from hESF decidualized for 3 and 14 days by treatment with oestradiol and medroxyprogesterone acetate. Cellular and whole endometrial/decidual tissue miR expression was quantified by qPCR and localized by in situ hybridization. The function of miR-19b-3p in HTR8/Svneo trophoblast cells was investigated using real time cell analysis (xCELLigence) and gene expression qPCR.
RESULTS
From our miR screen we found that essentially all hESF miR release was reduced following in vitro decidualization, significantly so for miR-17-5p, miR-21-3p, miR-34c-3p, miR-106b-5p, miR-138-5p, miR-296-5p, miR-323a-3p, miR-342-3p, miR-491-5p, miR-503-5p and miR-542-5p. qPCR demonstrated that miR-19b-3p, 181a-2-3p and miR-409-5p likewise showed a significant reduction in culture media following decidualization but no change was found in cellular miR expression following decidualization. hybridization localized miR-19b-3p to epithelial and stromal cells in the endometrium and qPCR identified that miR-19b-3p was significantly elevated in the cycling endometrium of patients with a history of early pregnancy loss compared to normally fertile controls. Functionally, overexpression of miR-19b-3p significantly reduced HTR8/Svneo trophoblast proliferation and increased HOXA9 expression.
DISCUSSION
Our data demonstrates that decidualization represses miR release by hESFs and overexpression of miR-19b-3p was found in endometrial tissue from patients with a history of early pregnancy loss. miR-19b-3p impaired HTR8/Svneo proliferation implying a role in trophoblast function. Overall we speculate that miR release by hESF may regulate other cell types within the decidua and that appropriate release of miRs by decidualized hESF is essential for healthy implantation and placentation.
简介
健康妊娠需要成功的囊胚着床到充分准备或“接受性”的子宫内膜。子宫子宫内膜基质成纤维细胞(hESF)的蜕膜化对于建立健康的妊娠至关重要。microRNAs(miRs)是细胞功能的关键调节剂,它们可以由供体细胞释放出来,影响受体细胞的生理状态。我们旨在确定蜕膜化如何影响 hESF 的 miR 释放,并研究了一种已被证明与复发性妊娠丢失相关的蜕膜化调节 miR,miR-19b-3p。
方法
通过用雌二醇和醋酸甲羟孕酮处理 hESF 使其蜕膜化 3 天和 14 天,通过 miR 微阵列测定 hESF 的 miR 释放。通过 qPCR 定量细胞和整个子宫内膜/蜕膜组织中的 miR 表达,并通过原位杂交进行定位。使用实时细胞分析(xCELLigence)和基因表达 qPCR 研究 miR-19b-3p 在 HTR8/Svneo 滋养层细胞中的功能。
结果
从我们的 miR 筛选中,我们发现 hESF 的几乎所有 miR 释放在体外蜕膜化后均减少,miR-17-5p、miR-21-3p、miR-34c-3p、miR-106b-5p、miR-138-5p、miR-296-5p、miR-323a-3p、miR-342-3p、miR-491-5p、miR-503-5p 和 miR-542-5p 明显减少。qPCR 表明,miR-19b-3p、181a-2-3p 和 miR-409-5p 同样在蜕膜化后培养基中的表达显著降低,但蜕膜化后细胞中的 miR 表达没有变化。杂交将 miR-19b-3p 定位到子宫内膜中的上皮和基质细胞,qPCR 确定与正常生育对照相比,有早期妊娠丢失史的患者的循环子宫内膜中 miR-19b-3p 显著升高。功能上,miR-19b-3p 的过表达显著降低了 HTR8/Svneo 滋养层细胞的增殖,并增加了 HOXA9 的表达。
讨论
我们的数据表明,蜕膜化抑制 hESF 的 miR 释放,并且在有早期妊娠丢失史的患者的子宫内膜组织中发现 miR-19b-3p 过表达。miR-19b-3p 损害了 HTR8/Svneo 的增殖,暗示其在滋养层功能中的作用。总体而言,我们推测 hESF 的 miR 释放可能调节蜕膜中的其他细胞类型,并且蜕膜化的 hESF 适当释放 miR 对于健康的着床和胎盘形成至关重要。
Zotero 插件