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本文引用的文献

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Role of Cdx2 and cell polarity in cell allocation and specification of trophectoderm and inner cell mass in the mouse embryo.Cdx2和细胞极性在小鼠胚胎滋养外胚层和内细胞团的细胞分配及特化中的作用。
Genes Dev. 2008 Oct 1;22(19):2692-706. doi: 10.1101/gad.486108.
2
Blastomeres of the mouse embryo lose totipotency after the fifth cleavage division: expression of Cdx2 and Oct4 and developmental potential of inner and outer blastomeres of 16- and 32-cell embryos.小鼠胚胎的卵裂球在第五次卵裂后丧失全能性:Cdx2和Oct4的表达以及16细胞和32细胞胚胎内、外卵裂球的发育潜能。
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Computer simulation of emerging asymmetry in the mouse blastocyst.小鼠囊胚中出现的不对称性的计算机模拟。
Development. 2008 Apr;135(8):1407-14. doi: 10.1242/dev.014555.
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Formation of the embryonic-abembryonic axis of the mouse blastocyst: relationships between orientation of early cleavage divisions and pattern of symmetric/asymmetric divisions.小鼠囊胚胚胎-反胚胎轴的形成:早期卵裂分裂方向与对称/不对称分裂模式之间的关系。
Development. 2008 Mar;135(5):953-62. doi: 10.1242/dev.014316. Epub 2008 Jan 30.
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Spatial alignment of the mouse blastocyst axis across the first cleavage plane is caused by mechanical constraint rather than developmental bias among blastomeres.小鼠囊胚轴在第一次卵裂平面上的空间排列是由机械约束而非卵裂球之间的发育偏向引起的。
Mol Reprod Dev. 2008 Jul;75(7):1143-53. doi: 10.1002/mrd.20856.
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Cdx2 acts downstream of cell polarization to cell-autonomously promote trophectoderm fate in the early mouse embryo.Cdx2在细胞极化下游发挥作用,以细胞自主方式促进小鼠早期胚胎滋养外胚层命运的形成。
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Stochastic patterning in the mouse pre-implantation embryo.小鼠植入前胚胎中的随机模式形成
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Blastocyst axis is specified independently of early cell lineage but aligns with the ZP shape.囊胚轴的指定独立于早期细胞谱系,但与透明带形状对齐。
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Histone arginine methylation regulates pluripotency in the early mouse embryo.组蛋白精氨酸甲基化调控小鼠早期胚胎的多能性。
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10
Allocation of cells in mouse blastocyst is not determined by the order of cleavage of the first two blastomeres.小鼠囊胚中的细胞分配并非由最初两个卵裂球的分裂顺序所决定。
Biol Reprod. 2006 Oct;75(4):582-7. doi: 10.1095/biolreprod.106.053165. Epub 2006 Jul 5.

超排卵对2细胞期CF1小鼠胚胎单个卵裂球形成囊胚的贡献的影响。

The effect of superovulation on the contributions of individual blastomeres from 2-cell stage CF1 mouse embryos to the blastocyst.

作者信息

Katayama Mika, Roberts R Michael

机构信息

Division of Animal Sciences, Christopher S. Bond Life Sciences Center, University of Missouri, Columbia, MO 65211, USA.

出版信息

Int J Dev Biol. 2010;54(4):675-81. doi: 10.1387/ijdb.092942mk.

DOI:10.1387/ijdb.092942mk
PMID:20209440
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9040203/
Abstract

It remains controversial whether blastomeres of 2-cell stage mouse embryos show bias in their contribution to the blastocyst and whether there is any effect of superovulation. Two-cell stage embryos from CF1 mice were derived by either natural breeding (N) or superovulation (S) and cultured in vitro. At blastocyst, inner cell mass and trophectoderm were distinguished by Cdx2 and Oct4 immunostaining. A fluorescent dye (CM-Dil) was also used to tag individual blastomeres at the 2-cell stage, and the descendant cells identified by their red fluorescence. S and N embryos developed to blastocyst at the same rate and contained a similar number of cells. However, with S embryos, the descendants of the blastomere labeled with CM-DiI contributed predominantly to either the embryonic or abembryonic pole about 70% of the time, whereas most N embryos displayed random patterning, with no restriction to one or other of the poles. In S-embryos, but not N-embryos, the leading blastomere at second cleavage contributed preferentially to the embryonic pole of the blastocyst and the lagging blastomere to the abembryonic pole and hence mural trophectoderm. In addition, a tetrahedral rather than a flat morphology at the 4-cell stage of S-embryos was strongly biased to displaying the embryonic/abembryonic pattern at blastocyst. In contrast, S-embryos lacking a zona pellucida resembled N embryos in their patterning. In CF1 mice, superovulation has little effect on development to blastocyst, but enforces a greater degree of lineage restriction than natural breeding, most likely through constraints imposed by the zona pellucida.

摘要

2细胞期小鼠胚胎的卵裂球在对囊胚的贡献上是否存在偏向,以及超排卵是否有任何影响,这仍然存在争议。通过自然交配(N)或超排卵(S)获得CF1小鼠的2细胞期胚胎,并进行体外培养。在囊胚期,通过Cdx2和Oct4免疫染色区分内细胞团和滋养外胚层。还使用一种荧光染料(CM-Dil)在2细胞期标记单个卵裂球,并通过其红色荧光识别后代细胞。S组和N组胚胎发育到囊胚的速率相同,且细胞数量相似。然而,对于S组胚胎,用CM-DiI标记的卵裂球的后代在约70%的时间里主要分布在胚胎极或反胚胎极,而大多数N组胚胎呈现随机分布,对两极中的任何一极都没有限制。在S组胚胎中,但不在N组胚胎中,第二次分裂时的领先卵裂球优先分布到囊胚的胚胎极,而落后的卵裂球分布到反胚胎极,进而分布到壁滋养外胚层。此外,S组胚胎在4细胞期呈四面体而非扁平形态,这强烈倾向于在囊胚期呈现胚胎/反胚胎模式。相比之下,缺乏透明带的S组胚胎在其分布模式上与N组胚胎相似。在CF1小鼠中,超排卵对发育到囊胚的影响很小,但比自然交配施加了更大程度的谱系限制,这很可能是由于透明带施加的限制。