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从诊断为神经管缺陷的羊水样本中分离人神经干细胞。

Isolation of Human Neural Stem Cells from the Amniotic Fluid with Diagnosed Neural Tube Defects.

作者信息

Chang Yu-Jen, Su Hong-Lin, Hsu Lee-Feng, Huang Po-Jui, Wang Tzu-Hao, Cheng Fu-Chou, Hsu Li-Wen, Tsai Ming-Song, Chen Chih-Ping, Chang Yao-Lung, Chao An-Shine, Hwang Shiaw-Min

机构信息

1 Bioresource Collection and Research Center, Food Industry Research and Development Institute , Hsinchu, Taiwan .

2 Department of Life Sciences, National Chung-Hsing University , Taichung, Taiwan .

出版信息

Stem Cells Dev. 2015 Aug 1;24(15):1740-50. doi: 10.1089/scd.2014.0516. Epub 2015 Jun 4.

Abstract

Human neural stem cells (NSCs) are particularly valuable for the study of neurogenesis process and have a therapeutic potential in treating neurodegenerative disorders. However, current progress in the use of human NSCs is limited due to the available NSC sources and the complicated isolation and culture techniques. In this study, we describe an efficient method to isolate and propagate human NSCs from the amniotic fluid with diagnosed neural tube defects (NTDs), specifically, anencephaly. These amniotic fluid-derived NSCs (AF-NSCs) formed neurospheres and underwent long-term expansion in vitro. In addition, these cells showed normal karyotypes and telomerase activity and expressed NSC-specific markers, including Nestin, Sox2, Musashi-1, and the ATP-binding cassette G2 (ABCG2). AF-NSCs displayed typical morphological patterns and expressed specific markers that were consistent with neurons, astrocytes, oligodendrocytes, and dopaminergic neurons after proper induction conditions. Furthermore, grafted AF-NSCs improved the physiological functions in a rat stroke model. The ability to isolate and bank human NSCs from this novel source provides a unique opportunity for translational studies of neurological disorders.

摘要

人类神经干细胞(NSCs)对于神经发生过程的研究特别有价值,并且在治疗神经退行性疾病方面具有治疗潜力。然而,由于可用的神经干细胞来源以及复杂的分离和培养技术,目前人类神经干细胞的应用进展有限。在本研究中,我们描述了一种从诊断为神经管缺陷(NTDs)、特别是无脑畸形的羊水样本中分离和扩增人类神经干细胞的有效方法。这些羊水来源的神经干细胞(AF-NSCs)形成了神经球并在体外进行了长期扩增。此外,这些细胞显示出正常的核型和端粒酶活性,并表达神经干细胞特异性标志物,包括巢蛋白(Nestin)、性别决定区Y框蛋白2(Sox2)、神经细胞黏附分子(Musashi-1)和ATP结合盒转运体G2(ABCG2)。在适当的诱导条件下,AF-NSCs表现出典型的形态模式,并表达与神经元、星形胶质细胞、少突胶质细胞和多巴胺能神经元一致的特异性标志物。此外,移植的AF-NSCs改善了大鼠中风模型的生理功能。从这个新来源分离和保存人类神经干细胞的能力为神经疾病的转化研究提供了独特的机会。

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