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Epigenetic regulator function through mouse gastrulation

原肠化 表观遗传学 生物 突变体 表型 染色质 转录调控 细胞生物学 计算生物学 转录因子 遗传学 胚胎干细胞 基因
作者
Stefanie Grosswendt,Helene Kretzmer,Zachary D. Smith,Abhishek Sampath Kumar,Sara Hetzel,Lars Wittler,Sven Klages,Bernd Timmermann,Shankar Mukherji,Alexander Meissner
出处
期刊:Nature [Springer Nature]
卷期号:584 (7819): 102-108 被引量:112
标识
DOI:10.1038/s41586-020-2552-x
摘要

During ontogeny, proliferating cells become restricted in their fate through the combined action of cell-type-specific transcription factors and ubiquitous epigenetic machinery, which recognizes universally available histone residues or nucleotides in a context-dependent manner1,2. The molecular functions of these regulators are generally well understood, but assigning direct developmental roles to them is hampered by complex mutant phenotypes that often emerge after gastrulation3,4. Single-cell RNA sequencing and analytical approaches have explored this highly conserved, dynamic period across numerous model organisms5–8, including mouse9–18. Here we advance these strategies using a combined zygotic perturbation and single-cell RNA-sequencing platform in which many mutant mouse embryos can be assayed simultaneously, recovering robust morphological and transcriptional information across a panel of ten essential regulators. Deeper analysis of central Polycomb repressive complex (PRC) 1 and 2 components indicates substantial cooperativity, but distinguishes a dominant role for PRC2 in restricting the germline. Moreover, PRC mutant phenotypes emerge after gross epigenetic and transcriptional changes within the initial conceptus prior to gastrulation. Our experimental framework may eventually lead to a fully quantitative view of how cellular diversity emerges using an identical genetic template and from a single totipotent cell. An experimental and analytical pipeline is used to assess, at the single-cell level, complex transcriptional and morphological mutant phenotypes that occur in mouse embryos during gastrulation.
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