Generation of germinal-vesicle oocytes from mouse embryonic stem cells under an ovarian soma-free condition (EM-Seq)
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https://www.ncbi.nlm.nih.gov/geo/query/acc.cgi?acc=GSE272449
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In vitro oogenesis provides a platform to elucidate the mechanism of oocyte development and advance reproductive medicine. The prevalent in vitro oogenesis model requires ovarian somatic cells (OSCs) to support oocyte development, yet complex three-dimensional oocyte–OSC interactions pose difficulties in systems regulation and mechanistic understanding. Here, we present an OSC-free system of in vitro oogenesis: upon optimized provision of retinoic acid and bone morphogenetic protein on feeders, mouse primordial germ cell-like cells induced from embryonic stem cells propagate robustly, and enter/progress through meiotic prophase I, generating abundant fetal oocyte-like cells at diplotene arrest. With key cytokines, signaling activators, and antioxidants, they show prominent growth and differentiate into cells comparable to germinal-vesicle oocytes in morphology, transcriptome, and histone-modification profiles, with competence to resume meiosis with germinal-vesicle breakdown. By reconstituting major phases of oogenesis with minimal components, our study creates a foundation for OSC-free in vitro oogenesis in mammals, including humans. Transcriptome analysis of pre-antral oocytes from mouse embryonic stem cells under an ovarian soma-free condition
创建时间:
2025-08-18



