A Simplified Method for Ultra-Low Density, Long-Term Primary Hippocampal Neuron Culture

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Neuroscienze

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Neuroscienze

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JoVE Journal Neuroscienze

A Simplified Method for Ultra-Low Density, Long-Term Primary Hippocampal Neuron Culture

DOI:

10.3791/53797-v

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11:19 min

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March 05, 2016

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Zhongming Lu*^1,2, Mariel Piechowicz*¹, Shenfeng Qiu

¹Department of Basic Medical Sciences,University of Arizona College of Medicine-Phoenix, ²Jiangsu Provincial Center for Disease Control and Prevention

Capitoli

00:05Titolo
00:5924-well Plate Preparation for High and Low Density Neuron Culture
01:48Brain Removal and Hippocampi Dissection of E16.5 – E17.5 Mouse Embryos
04:02Enzymatic Digestion and Separation into Single Neurons
06:53Plating of Neurons and Long Term Co-Culture
08:51Results: Experimental Manipulations of Low Density Neurons Grown in Co-Culture
10:23Conclusion

Summary

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Low density cultures of primary hippocampal neurons usually require glia feeder layer to supply neurotrophic factors and sustain longevity. We describe here a simplified method to culture ultra-low density neurons on glass coverslips in the presence of a high density neuronal feeder layer, which facilitates investigation of specific neuronal-autonomous mechanisms.

A Simplified Method for Ultra-Low Density, Long-Term Primary Hippocampal Neuron Culture

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