4.7 Article

Cellular, subcellular and functional in vivo labeling of the spinal cord using vital dyes

Journal

NATURE PROTOCOLS
Volume 8, Issue 3, Pages 481-490

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/nprot.2013.022

Keywords

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Funding

  1. European Research Council (ERC)
  2. Deutsche Forschungsgemeinschaft (DFG) [Sonderforschungsbereiche (SFB) 571, SFB 870, SFB-Tr 128]
  3. German Federal Ministry of Research and Education (Competence Network Multiple Sclerosis)
  4. Verein Therapieforschung fur MS-Kranke e.V.
  5. Institute of Advanced Studies (Technische Universitat Munchen)
  6. Alexander von Humboldt Foundation
  7. Center for Integrated Protein Science (Munich)
  8. DFG [SFB 596]
  9. German Center for Neurodegenerative Disease (DZNE Munich)
  10. national funding agency ('Bundesministerium fur Bildung und Forschung')
  11. DANA foundation
  12. Graduate School of Technische Universitat Munchen (TUM-GS)

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Here we provide a protocol for rapidly labeling different cell types, distinct subcellular compartments and key injury mediators in the spinal cord of living mice. This method is based on the application of synthetic vital dyes to the surgically exposed spinal cord. Suitable vital dyes applied in appropriate concentrations lead to reliable in vivo labeling, which can be combined with genetic tags and in many cases preserved for postfixation analysis. In combination with in vivo imaging, this approach allows the direct observation of central nervous system physiology and pathophysiology at the cellular, subcellular and functional level. Surgical exposure and preparation of the spinal cord can be achieved in less than 1 h, and then dyes need to be applied for 30-60 min before the labeled spinal cord can be imaged for several hours.

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