Minimum neuron density for synchronized bursts in a rat cortical culture on multi-electrode arrays

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• 作者：D. Ito ; H. Tamate ; M. Nagayama ; T. Uchida ; S.N. Kudoh ; K. Gohara
• 关键词：dissociated culture ; neuronal network ; immunocytochemistry ; fluorescence microscopy ; neuronal survival
• 刊名：Neuroscience
• 出版年：2010
• 出版时间：24 November 2010
• 年：2010
• 卷：171
• 期：1
• 页码：50-61
• 全文大小：1499 K

文摘

To investigate the minimum neuron and neurite densities required for synchronized bursts, we cultured rat cortical neurons on planar multi-electrode arrays (MEAs) at five plating densities (2500, 1000, 500, 250, and 100 cells/mm²) using two culture media: Neuron Culture Medium and Dulbecco's Modified Eagle Medium supplemented with serum (DMEM/serum). Long-term recording of spontaneous electrical activity clarified that the cultures exhibiting synchronized bursts required an initial plating density of at least 250 cells/mm² for Neuron Culture Medium and 500 cells/mm² for DMEM/serum. Immediately after electrical recording, immunocytochemistry of microtubule-associated protein 2 (MAP2) and Neurofilament 200 kD (NF200) was performed directly on MEAs to investigate the actual densities of neurons and neurites forming the networks. Immunofluorescence observation revealed that the construction of complicated neuronal networks required the same initial plating density as for synchronized bursts, and that overly sparse cultures showed significant decreases of neurons and neurites. We also found that the final densities of surviving neurons at 1 month decreased greatly compared with the initial plating densities and became saturated in denser cultures. In addition, the area of neurites and the number of nuclei were saturated in denser cultures. By comparing both the results of electrophysiological recording and immunocytochemical observation, we revealed that there is a minimum threshold of neuron densities that must be met for the exhibition of synchronized bursts. Interestingly, these minimum densities of MAP2-positive final neurons did not differ between the two culture media; the density was approximately 50 neurons/mm². This value was obtained in the cultures with the initial plating densities of 250 cells/mm² for Neuron Culture Medium and 500 cells/mm² for DMEM/serum.