Published: Vol 3, Iss 15, Aug 5, 2013 DOI: 10.21769/BioProtoc.842 Views: 11518
Reviewed by: Lin FangFanglian HeAnonymous reviewer(s)
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Abstract
This protocol describes how to visualize neuronal morphology and how to determine neuronal complexity of immature and mature hippocampal neurons in the mouse in vivo including tissue preparation, staining of brain sections and confocal cell analysis.
Materials and Reagents
Equipment
Software
Procedure
Representative data
Figure 2. Light microscope (A) and confocal microscope picture (B) of Golgi stained neurons. Picture shown in B (left panel) was used for image analysis with Amira (right panel).
Recipes
NaCl | 160 g/L |
Na2HPO4 | 23 g/L |
NaH2PO4 | 28.84 g/L |
KCl | 4 g/L |
KH2PO4 | 4 g/L |
Trizma base | 24.23 g/L |
NaCl | 80.06 g/L |
TBS | 100 ml |
Horse serum | 3 ml |
Triton X-100 | 0.25 ml |
NaH2PO4.H2O | 13.9 g/500 ml |
0.2 M Dibasic Stock | |
Na2HPO4.7H2O | 53.65 g/L |
0.2 M Monobasic Stock | 0.2 M Dibasic Stock | pH |
57 ml | 243 ml | 7.4 |
Gelatine | 1.5 g |
Chromium (III) potassium sulfate dodecahydrate | 0.25 g |
1x PBS | 40 ml | |
Mowiol | 10 g | → stir for 24 h |
Add Glycerol | 20 ml | → stir for 24 h |
Acknowledgments
This protocol is adapted from Seib et al. (2012).
References
Article Information
Copyright
© 2013 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Seib, D. R. M. and Martin-Villalba, A. (2013). Neuronal Morphology Analysis. Bio-protocol 3(15): e842. DOI: 10.21769/BioProtoc.842.
Category
Neuroscience > Neuroanatomy and circuitry > Live-cell imaging
Stem Cell > Adult stem cell > Neural stem cell
Cell Biology > Tissue analysis > Tissue isolation
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