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子宫颈和子宫缺乏雌激素受体α的雌性小鼠的胚胎滞留。

Oviductal Retention of Embryos in Female Mice Lacking Estrogen Receptor α in the Isthmus and the Uterus.

机构信息

School of Molecular Biosciences, Center for Reproductive Biology, College of Veterinary Medicine, Washington State University, Pullman, Washington, US.

Reproductive and Developmental Biology Laboratory, National Institute of Environmental Health Sciences, National Institutes of Health (NIH/NIEHS), Department of Health and Human Services, Research Triangle Park, North Carolina, US.

出版信息

Endocrinology. 2020 Feb 1;161(2). doi: 10.1210/endocr/bqz033.

Abstract

Estrogen receptor α (ESR1; encoded by Esr1) is a crucial nuclear transcription factor for female reproduction and is expressed throughout the female reproductive tract. To assess the function of ESR1 in reproductive tissues without confounding effects from a potential developmental defect arising from global deletion of ESR1, we generated a mouse model in which Esr1 was specifically ablated during postnatal development. To accomplish this, a progesterone receptor Cre line (PgrCre) was bred with Esr1f/f mice to create conditional knockout of Esr1 in reproductive tissues (called PgrCreEsr1KO mice) beginning around 6 days after birth. In the PgrCreEsr1KO oviduct, ESR1 was most efficiently ablated in the isthmic region. We found that at 3.5 days post coitus (dpc), embryos were retrieved from the uterus in control littermates while all embryos were retained in the PgrCreEsr1KO oviduct. Additionally, serum progesterone (P4) levels were significantly lower in PgrCreEsr1KO compared to controls at 3.5 dpc. This finding suggests that expression of ESR1 in the isthmus and normal P4 levels allow for successful embryo transport from the oviduct to the uterus. Therefore, alterations in oviductal isthmus ESR1 signaling and circulating P4 levels could be related to female infertility conditions such as tubal pregnancy.

摘要

雌激素受体 α (ESR1; 由 Esr1 编码) 是女性生殖的关键核转录因子,在女性生殖道中广泛表达。为了评估 ESR1 在生殖组织中的功能而不受到 ESR1 全局缺失引起的潜在发育缺陷的混杂影响,我们生成了一种在出生后发育过程中特异性剔除 Esr1 的小鼠模型。为此,将孕激素受体 Cre 线 (PgrCre) 与 Esr1f/f 小鼠杂交,以在生殖组织中创建 Esr1 的条件性敲除 (称为 PgrCreEsr1KO 小鼠),大约从出生后 6 天开始。在 PgrCreEsr1KO 输卵管中,ESR1 在峡部区域被最有效地剔除。我们发现,在交配后 3.5 天 (dpc),对照同窝仔鼠的胚胎从子宫中取出,而所有胚胎都滞留在 PgrCreEsr1KO 输卵管中。此外,与对照组相比,PgrCreEsr1KO 在 3.5 dpc 时血清孕激素 (P4) 水平显著降低。这一发现表明,峡部的 ESR1 表达和正常的 P4 水平允许胚胎从输卵管成功运输到子宫。因此,输卵管峡部 ESR1 信号转导和循环 P4 水平的改变可能与输卵管妊娠等女性不孕情况有关。

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