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Culture of Mouse Embryonic Stem Cells with Serum but without Exogenous Growth Factors Is Sufficient to Generate Functional Hepatocyte-Like Cells

机译:具有血清但没有外源性生长因子的小鼠胚胎干细胞的培养足以产生功能性肝细胞样细胞

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摘要

Mouse embryonic stem cells (mESC) have been used to study lineage specification in vitro, including towards a hepatocyte-like fate, and such investigations guided lineage differentiation protocols for human (h)ESC. We recently described a four-step protocol to induce hepatocyte-like cells from hESC which also induced hepatocyte-like cell differentiation of mouse induced pluripotent stem cells. As ESC also spontaneously generate hepatocyte-like cells, we here tested whether the growth factors and serum used in this protocol are required to commit mESC and hESC to hepatocyte-like cells. Culture of mESC from two different mouse strains in the absence of serum and growth factors did not induce primitive streak/definitive endoderm genes but induced default differentiation to neuroectoderm on day 6. Although Activin-A and Wnt3 induced primitive streak/definitive endoderm transcripts most robustly in mESC, simple addition of serum also induced these transcripts. Expression of hepatoblast genes occurred earlier when growth factors were used for mESC differentiation. However, further maturation towards functional hepatocyte-like cells was similar in mESC progeny from cultures with serum, irrespective of the addition of growth factors, and irrespective of the mouse strain. This is in contrast to hESC, where growth factors are required for specification towards functional hepatocyte-like cells. Culture of mESC with serum but without growth factors did not induce preferential differentiation towards primitive endoderm or neuroectoderm. Thus, although induction of primitive streak/definitive endoderm specific genes and proteins is more robust when mESC are exposed to a combination of serum and exogenous growth factors, ultimate generation of hepatocyte-like cells from mESC occurs equally well in the presence or absence of exogenous growth factors. The latter is in contrast to what we observed for hESC. These results suggest that differences exist between lineage specific differentiation potential of mESC and hESC, requiring optimization of different protocols for ESC from either species.
机译:小鼠胚胎干细胞(mESC)已用于体外研究谱系规范,包括对肝细胞样命运的研究,此类研究指导了人类(h)ESC的谱系分化方案。我们最近描述了从hESC诱导肝细胞样细胞的四个步骤的协议,它还诱导小鼠诱导的多能干细胞的肝细胞样细胞分化。由于ESC还自发生成肝细胞样细胞,因此我们在此测试了该协议中使用的生长因子和血清是否需要将mESC和hESC提交至肝细胞样细胞。在没有血清和生长因子的情况下,来自两种不同小鼠品系的mESC的培养不会诱导原始条纹/定形内胚层基因,但是在第6天诱导了神经外胚层的默认分化。尽管Activin-A和Wnt3诱导原始条纹/定形内胚层的转录最有力。在mESC中,简单添加血清也会诱导这些转录本。当将生长因子用于mESC分化时,成肝细胞基因的表达较早发生。然而,无论是否添加生长因子,也不管小鼠品系,在具有血清的mESC后代中,向功能性肝细胞样细胞的进一步成熟都是相似的。这与hESC相反,在hESC中,生长因子是规范功能性肝细胞样细胞所必需的。用血清培养但没有生长因子的mESC不能诱导向原始内胚层或神经外胚层的优先分化。因此,尽管当mESC暴露于血清和外源性生长因子的组合下时,原始条纹/定形内胚层特异性基因和蛋白质的诱导作用更强,但是在存在或不存在外源性条件下,mESC最终产生类肝细胞的能力均相同生长因子。后者与我们观察到的hESC相反。这些结果表明,mESC和hESC的谱系特异性分化潜能之间存在差异,需要优化来自两种物种的ESC的不同方案。

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