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首页> 外文期刊>Molecular and Cellular Endocrinology >Retinoic acid induces parietal endoderm but not primitive endoderm and visceral endoderm differentiation in F9 teratocarcinoma stem cells with a targeted deletion of the Rex-1 (Zfp-42) gene.
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Retinoic acid induces parietal endoderm but not primitive endoderm and visceral endoderm differentiation in F9 teratocarcinoma stem cells with a targeted deletion of the Rex-1 (Zfp-42) gene.

机译:维甲酸可诱导F9畸胎癌干细胞的顶叶内胚层分化,但不诱导原始内胚层和内脏内胚层分化,并有针对性地缺失Rex-1(Zfp-42)基因。

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摘要

Cultured murine F9 teratocarcinoma stem cells resemble pluripotent stem cells of the inner cell mass of the mouse blastocyst and, depending upon their treatment, can be induced to differentiate along the primitive endoderm, the parietal endoderm (PE), or the visceral endoderm (VE) pathway. The Rex-1 gene encodes a zinc finger family transcription factor which is expressed at high levels in undifferentiated F9 stem cells, embryonic stem cells, and in other types of stem cells. To examine whether the Rex-1 protein plays a role in F9 cell differentiation, homologous recombination was employed to generate F9 cell lines which lack both alleles of Rex-1. F9 wild type cells in monolayer culture require both retinoic acid and cyclic AMP analogs to differentiate into PE, whereas the F9 Rex-1(-/-) cells differentiate into PE, as assessed by several molecular markers, including thrombomodulin and laminin B1, in the presence of RA alone. The F9 Rex-1(-/-) cells do not completely differentiate into VE after RA treatment in aggregate culture; they do not express alpha-fetoprotein, a definitive marker of VE differentiation. These results indicate that the Rex-1 transcription factor regulates the differentiation of F9 stem cells along several distinct cell lineages found in the early embryo.
机译:培养的鼠F9畸胎瘤干细胞类似于小鼠胚泡内部细胞团的多能干细胞,并且根据其治疗方法,可以诱导其沿原始内胚层,顶内胚层(PE)或内脏内胚层(VE)分化途径。 Rex-1基因编码一个锌指家族转录因子,该因子在未分化的F9干细胞,胚胎干细胞和其他类型的干细胞中高水平表达。为了检查Rex-1蛋白是否在F9细胞分化中起作用,采用同源重组产生缺少Rex-1两个等位基因的F9细胞系。单层培养中的F9野生型细胞既需要视黄酸又需要环状AMP类似物才能分化为PE,而F9 Rex-1(-/-)细胞则可以分化为PE,这是通过几种分子标志物评估的,包括血栓调节蛋白和层粘连蛋白B1。仅存在RA。在聚集培养中,RA处理后,F9 Rex-1(-/-)细胞不会完全分化为VE;它们不表达甲胎蛋白,这是VE分化的决定性标志。这些结果表明,Rex-1转录因子沿早期胚胎中发现的几种不同细胞谱系调节F9干细胞的分化。

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