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Generation of porcine endometrial organoids and their use as a model for enhancing embryonic attachment and elongation

胚胎 胚胎干细胞 基质凝胶 低温保存 滋养层 男科 细胞生物学 化学 类有机物 延伸率 胚胎发生 生物 细胞 胎盘 材料科学 生物化学 胎儿 极限抗拉强度 怀孕 医学 遗传学 冶金 基因
作者
Islam M. Saadeldin,A. Han,Seonggyu Bang,Heejae Kang,Heyyoung Kim,Mariam M. Abady,Ji‐Seon Jeong,Ha‐Jeong Kwon,Sanghoon Lee,Jongki Cho
出处
期刊:Reproduction [Bioscientifica]
卷期号:167 (2) 被引量:3
标识
DOI:10.1530/rep-23-0429
摘要

In brief Porcine endometrial organoids (EOs) were isolated and characterized, revealing distinctive features such as unique extracellular matrix formation, fusion into uterine bud-like structures, and facilitation of embryo elongation. The yield of EOs was significantly enhanced by cryopreservation medium supplemented with the rock inhibitor (Y-27632), resulting in reduced expression of apoptotic mRNAs and microRNAs. Abstract Endometrial organoids (EOs) are acceptable models for understanding maternal–embryonic cross talk. This study was conducted to generate EOs and optimize their cryopreservation and provide coculture modeling with embryos. The endometrial tissues were used for culturing the organoids inside domes of Matrigel ® . To improve the long-term storage of EOs, 10 µM ROCK inhibitor (RI) was added to the cryopreservation medium. Day 7 parthenogenetically activated embryos were cocultured with EOs or EO outgrowths, and embryonic cell numbers and embryo attachment were monitored. Spherical EOs 100–300 µm in size can be retrieved on day 7 of culture, and larger EOs, approximately 1.5 mm in diameter, can be maintained in the Matrigel ® dome for 21 days. The nuclear expression of Ki67 indicates that more than 80% of EOs nuclei were proliferative. EOs exhibit unique novel characters such as formation of extracellular matrix and ability for fusion. RI increased the yield and quality of organoids after freezing or thawing. The cell number of cocultured embryos increased five-fold, and the proportion of trophoblast outgrowths increased seven-fold compared with those of control embryos. The embryos cultured with EO-conditioned medium showed a better attachment rate than the other models, and – for the first time – we report embryonic elongation. Immunofluorescence staining of the attached embryos showed CDX2 in the periphery of EOs outgrowths. The 3D assembly and cryopreservation of EOs was optimized, and EO coculture supported embryo attachment, trophoblast outgrowth, and elongation, which would provide a valuable tool for studying the intricate processes involved in porcine embryo implantation.
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