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使用微流控芯片进行神经球的单细胞无酶解离。

Single-cell enzyme-free dissociation of neurospheres using a microfluidic chip.

机构信息

Institute of Biomedical Engineering and Nanomedicine, National Health Research Institutes , Zhunan, Miaoli 35053, Taiwan.

出版信息

Anal Chem. 2013 Dec 17;85(24):11920-8. doi: 10.1021/ac402724b. Epub 2013 Nov 22.

Abstract

Obtaining single dissociated cells from neurospheres is difficult using nonenzymatic methods. In this paper we report the development of a microfluidic-chip-based approach that utilizes flow and microstructures to dissociate neurospheres. We show that this microfluidic-chip-based neurosphere-dissociation method can generate high yields of single cells from dissociated neurospheres of mouse KT98 and DC115 cell models (passage number, 3-8; diameter range, 40-250 μm): 90% and 95%, respectively. The microfluidic-chip-dissociated cells had high viabilities (80-85%) and the ability to regrow into neurospheres, demonstrating the applicability of this device to neurosphere assay applications. In addition, the dissociated cells retained their normal differentiation potentials, as shown by their capabilities to differentiate into three neural lineages (neurons, astroglia, and oligodendrocytes) when cultured in differentiation culture conditions. Since this microfluidic-chip-based method does not require the use of enzymatic reagents, the risk of contamination from exogenous substances could be reduced, making it an attractive tool for a wide range of applications where neurosphere dissociation is needed.

摘要

用非酶法从神经球中获得单个解离细胞是困难的。本文报道了一种基于微流控芯片的方法,该方法利用流动和微结构来解离神经球。结果表明,该基于微流控芯片的神经球解离方法可以从分离的小鼠 KT98 和 DC115 细胞模型的神经球(传代数 3-8;直径范围 40-250μm)中获得高产率的单细胞:分别为 90%和 95%。微流控芯片解离的细胞具有较高的活力(80-85%),并且能够重新生长成神经球,表明该装置适用于神经球测定应用。此外,解离细胞保留了其正常的分化潜能,当在分化培养条件下培养时,其能够分化为三种神经谱系(神经元、星形胶质细胞和少突胶质细胞)。由于这种基于微流控芯片的方法不需要使用酶试剂,因此可以降低外源性物质污染的风险,使其成为需要神经球解离的广泛应用的有吸引力的工具。

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