Brain Dissection and Embedding for Organotypic Slice Culture
6:40
Vibratome Sectioning and Slice Culture
8:47
Ime-lapse Imaging
10:30
Results: Migration Behavior of Bcl11a Mutant Upper-layer Cortical Neurons
12:40
Conclusion
副本
The overall goal of this procedure is to directly observe radially migrating neurons in organotypic slice culture prepared from electroporated embryonic brain by time-lapse confocal microscopy. This method can help study key aspects of neocortex d
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This protocol provides instructions for direct observation of radially migrating cortical neurons. In utero electroporation, organotypic slice culture, and time-lapse confocal imaging are combined to directly and dynamically study the effects of overexpression or downregulation of genes of interest in migrating neurons and to analyze their differentiation during development.