首页> 外文期刊>Iranian Journal of Reproductive Medicine >THE EFFECT OF MOUSE EMBRYONIC FIBROBLAST IN DIRECT DIFFERENTIATION OF MOUSE EMBRYONIC STEM CELLS
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THE EFFECT OF MOUSE EMBRYONIC FIBROBLAST IN DIRECT DIFFERENTIATION OF MOUSE EMBRYONIC STEM CELLS

机译:小鼠胚胎成纤维细胞在小鼠胚胎干细胞直接分化中的作用

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Background: Since embryonic stem (ES) cells have the dual ability to proliferate indefinitely and differentiate into multiple tissue types, ES cells could potentially provide an unlimited cell supply for human transplantation.Objective: In order to study the differentiation of mouse embryonic stem (mES) cells, they were cultured in suspension by using ES media without Leukemia Inhibitory Factor (LIF) to induce spontaneous differentiation. Cellular morphology of differentiated derivatives was then evaluated.Materials and Methods: Undifferentiated mES from our laboratory were cultured in three different settings by using ES media containing 0.1% / 1mM trypsin/EDTA and removing LIF; in the absence of murine embryonic fibroblast (MEF) feeder cells (group 1), in the presence of MEF feeder cells with a density of 0.5?—105 cells/ml (group 2), and 0.5?—106 cells/ml (group 3). Five days after the initiation of cell culture, and inducing mES cells to form embryoid bodies (EBs), they were removed from dish by centrifugation, and then they were cultured on collagen coated dishes for 20 days. The dishes were fixed and stained by Wright-Gimsa method at the end of the study period.Results: In group 1, mES cells showed spontaneous differentiation to all derivatives of three germ cells, including: epithelia like, fibroblast like and neron-like cells. In group 2, almost all ES cells were found to be differentiated into granular progenitor cells including hematopoietic cell lineages. In group 3, various morphologies including nerve cell lineages and fibroblastlike cells were detected.Conclusion: Differentiation of mES cells can be a dose response process, depending on the factors that may be released from MEF feeder layer to ES media in a coculture system. Our results indicated that in the presence of low numbers of MEF cells, mES cells can spontaneously differentiate into hematopoeitic cell lineages.
机译:背景:由于胚胎干(ES)细胞具有无限增殖和分化为多种组织类型的双重能力,因此ES细胞可能为人类移植提供无限的细胞供应。目的:为了研究小鼠胚胎干(mES)的分化)细胞,使用不含白血病抑制因子(LIF)的ES培养基悬浮培养,以诱导自发分化。材料和方法:通过使用含有0.1%/ 1mM胰蛋白酶/ EDTA的ES培养基并去除LIF,在三种不同的环境下培养来自我们实验室的未分化mES。在没有鼠胚胎成纤维细胞(MEF)饲养细胞的情况下(组1),在有MEF饲养细胞的密度为0.5?-105细胞/ ml(组2)和0.5?-106细胞/ ml(组3)。在开始细胞培养并诱导mES细胞形成类胚体(EB)后五天,通过离心将它们从培养皿中取出,然后在胶原蛋白包被的培养皿中培养20天。结果:在第1组中,mES细胞自发分化为三种生殖细胞的所有衍生物,包括:上皮样,成纤维细胞样和神经元样细胞。 。在第2组中,几乎所有ES细胞都被分化为粒状祖细胞,包括造血细胞谱系。在第3组中,检测到各种形态,包括神经细胞谱系和成纤维细胞样细胞。结论:取决于在共培养系统中从MEF饲养层释放到ES培养基的因素,mES细胞的分化可能是一个剂量反应过程。我们的结果表明,在存在少量MEF细胞的情况下,mES细胞可以自发分化为造血细胞谱系。

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