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如何在微电极阵列(MEA)上培养、记录和刺激神经网络。

How to culture, record and stimulate neuronal networks on micro-electrode arrays (MEAs).

作者信息

Hales Chadwick M, Rolston John D, Potter Steve M

机构信息

Department of Neurology, Emory University School of Medicine, USA.

出版信息

J Vis Exp. 2010 May 30(39):2056. doi: 10.3791/2056.

Abstract

For the last century, many neuroscientists around the world have dedicated their lives to understanding how neuronal networks work and why they stop working in various diseases. Studies have included neuropathological observation, fluorescent microscopy with genetic labeling, and intracellular recording in both dissociated neurons and slice preparations. This protocol discusses another technology, which involves growing dissociated neuronal cultures on micro-electrode arrays (also called multi-electrode arrays, MEAs). There are multiple advantages to using this system over other technologies. Dissociated neuronal cultures on MEAs provide a simplified model in which network activity can be manipulated with electrical stimulation sequences through the array's multiple electrodes. Because the network is small, the impact of stimulation is limited to observable areas, which is not the case in intact preparations. The cells grow in a monolayer making changes in morphology easy to monitor with various imaging techniques. Finally, cultures on MEAs can survive for over a year in vitro which removes any clear time limitations inherent with other culturing techniques. Our lab and others around the globe are utilizing this technology to ask important questions about neuronal networks. The purpose of this protocol is to provide the necessary information for setting up, caring for, recording from and electrically stimulating cultures on MEAs. In vitro networks provide a means for asking physiologically relevant questions at the network and cellular levels leading to a better understanding of brain function and dysfunction.

摘要

在过去的一个世纪里,世界各地的许多神经科学家毕生致力于了解神经元网络如何工作以及它们在各种疾病中为何停止工作。研究包括神经病理学观察、基因标记荧光显微镜检查以及在解离神经元和脑片标本中的细胞内记录。本方案讨论了另一种技术,即在微电极阵列(也称为多电极阵列,MEA)上培养解离的神经元培养物。与其他技术相比,使用该系统有多个优点。MEA上的解离神经元培养物提供了一个简化的模型,其中网络活动可以通过阵列的多个电极用电刺激序列进行操纵。由于网络较小,刺激的影响仅限于可观察区域,而在完整标本中则并非如此。细胞以单层生长,便于用各种成像技术监测形态变化。最后,MEA上的培养物在体外可以存活一年以上,这消除了其他培养技术固有的明显时间限制。我们实验室和全球其他实验室正在利用这项技术来研究有关神经元网络的重要问题。本方案的目的是提供建立、护理、记录和电刺激MEA上的培养物所需的信息。体外网络提供了一种在网络和细胞水平上提出生理相关问题的方法,从而更好地理解脑功能和功能障碍。

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