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基于琼脂糖凝胶的神经球培养系统可在体外富集神经元谱系细胞。

An agarose gel-based neurosphere culture system leads to enrichment of neuronal lineage cells in vitro.

作者信息

Park Kyuhee, Nam Yeonju, Choi Yongmun

机构信息

Gyeonggi Bio-Center, Gyeonggi Institute of Science and Technology Promotion, Suwon, Gyeonggi-do, 443-270, South Korea.

出版信息

In Vitro Cell Dev Biol Anim. 2015 May;51(5):455-62. doi: 10.1007/s11626-014-9855-x. Epub 2014 Dec 25.

DOI:10.1007/s11626-014-9855-x
PMID:25539864
Abstract

Stem cell-based therapy holds great potential especially for neurological disorders. However, clinical applications await further understanding of many aspects of stem cell differentiation and development of technology enabling manipulation of stem cells into desired cell types in the central nervous system. Here, we developed a new method that leads to enrichment of neuronal lineage cells in neural stem cell cultures. The protocol involves cultivation of primary cells derived from the forebrains of rat E18 embryos above a layer of nonadhesive hard agarose gel in the form of neurospheres. In contrast to the neurospheres that were cultured above an anti-adhesive hydrogel layer, the primary cells that were cultured above a layer of agarose gel preferentially differentiated into β-III tubulin-positive neurons when allowed to undergo differentiation in vitro.In an effort to investigate the mechanism behind this observation, we found that the gene expression of a vertebrate neuronal determination gene (neurogenin1) was enhanced in the neurospheres that proliferated above a layer of agarose gel as compared with the control, and the gene expression level of neurogenin1 was quite well correlated with the rigidity of agarose gel. These results indicate that agarose gel can contribute, at least in part, to enrich neuronal progenitors and immature postmitotic neurons during neurosphere formation and may provide additional information to establish efficient protocols for the neural stem cell-based study.

摘要

基于干细胞的疗法具有巨大潜力,尤其对于神经疾病而言。然而,临床应用尚有待进一步了解干细胞分化的诸多方面,并有待开发能够将干细胞操控为中枢神经系统中所需细胞类型的技术。在此,我们开发了一种新方法,可在神经干细胞培养物中富集神经谱系细胞。该方案包括将源自大鼠E18胚胎前脑的原代细胞培养成神经球形式,置于一层非粘附性硬琼脂糖凝胶之上。与培养在抗粘附水凝胶层之上的神经球相比,培养在琼脂糖凝胶层之上的原代细胞在体外进行分化时优先分化为β-III微管蛋白阳性神经元。为了探究这一观察结果背后的机制,我们发现与对照组相比,在琼脂糖凝胶层之上增殖的神经球中,一种脊椎动物神经决定基因(神经生成素1)的基因表达增强,且神经生成素1的基因表达水平与琼脂糖凝胶的硬度密切相关。这些结果表明,琼脂糖凝胶至少在一定程度上有助于在神经球形成过程中富集神经祖细胞和未成熟的有丝分裂后神经元,并可能为建立基于神经干细胞的研究的有效方案提供额外信息。

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