Maternally and zygotically provided Cdx2 have novel and critical roles for early development of the mouse embryo

生物 细胞生物学 胚泡 内细胞团 合子 卵裂球 胚胎 CDX2 细胞命运测定 滋养层 胚胎干细胞 胚胎发生 遗传学 转录因子 基因 胎盘 同源盒 胎儿 怀孕
作者
Agnieszka Jędrusik,Alexander W. Bruce,Meng How Tan,Denise Leong,Maria Skamagki,Mylene Yao,Magdalena Zernicka‐Goetz
出处
期刊:Developmental Biology [Elsevier]
卷期号:344 (1): 66-78 被引量:80
标识
DOI:10.1016/j.ydbio.2010.04.017
摘要

Divisions of polarised blastomeres that allocate polar cells to outer and apolar cells to inner positions initiate the first cell fate decision in the mouse embryo. Subsequently, outer cells differentiate into trophectoderm while inner cells retain pluripotency to become inner cell mass (ICM) of the blastocyst. Elimination of zygotic expression of trophectoderm-specific transcription factor Cdx2 leads to defects in the maintenance of the blastocyst cavity, suggesting that it participates only in the late stage of trophectoderm formation. However, we now find that mouse embryos also have a maternally provided pool of Cdx2 mRNA. Moreover, depletion of both maternal and zygotic Cdx2 from immediately after fertilization by three independent approaches, dsRNAi, siRNAi and morpholino oligonucleotides, leads to developmental arrest at much earlier stages than expected from elimination of only zygotic Cdx2. This developmental arrest is associated with defects in cell polarisation, reflected by expression and localisation of cell polarity molecules such as Par3 and aPKC and cell compaction at the 8- and 16-cell stages. Cells deprived of Cdx2 show delayed development with increased cell cycle length, irregular cell division and increased incidence of apoptosis. Although some Cdx2-depleted embryos initiate cavitation, the cavity cannot be maintained. Furthermore, expression of trophectoderm-specific genes, Gata3 and Eomes, and also the trophectoderm-specific cytokeratin intermediate filament, recognised by Troma1, are greatly reduced or undetectable. Taken together, our results indicate that Cdx2 participates in two steps leading to trophectoderm specification: appropriate polarisation of blastomeres at the 8- and 16-cell stage and then the maintenance of trophectoderm lineage-specific differentiation.
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