4.4 Article

Two-photon Imaging of Cellular Dynamics in the Mouse Spinal Cord

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出版社

JOURNAL OF VISUALIZED EXPERIMENTS
DOI: 10.3791/52580

关键词

Neuroscience; Issue 96; spinal cord; two-photon microscopy; ex vivo; transplantation; cellular dynamics; axons; neural precursor cells; remyelination; neuroinflammation

资金

  1. National Institutes of Health (NIH) [R01 GM-41514, R39 GM-048071, R01 NS-074987]
  2. National Multiple Sclerosis Society (NMSS) Collaborative Center Research Award [CA1058-A-8]
  3. NMSS Grant [RG4925]
  4. NIH Training Grant [T32-AI-060573]
  5. NMSS Postdoctoral Fellowship [FG 1960-A-1]
  6. George E. Hewitt Foundation for Medical Research

向作者/读者索取更多资源

Two-photon (2P) microscopy is utilized to reveal cellular dynamics and interactions deep within living, intact tissues. Here, we present a method for live-cell imaging in the murine spinal cord. This technique is uniquely suited to analyze neural precursor cell (NPC) dynamics following transplantation into spinal cords undergoing neuroinflammatory demyelinating disorders. NPCs migrate to sites of axonal damage, proliferate, differentiate into oligodendrocytes, and participate in direct remyelination. NPCs are thereby a promising therapeutic treatment to ameliorate chronic demyelinating diseases. Because transplanted NPCs migrate to the damaged areas on the ventral side of the spinal cord, traditional intravital 2P imaging is impossible, and only information on static interactions was previously available using histochemical staining approaches. Although this method was generated to image transplanted NPCs in the ventral spinal cord, it can be applied to numerous studies of transplanted and endogenous cells throughout the entire spinal cord. In this article, we demonstrate the preparation and imaging of a spinal cord with enhanced yellow fluorescent protein-expressing axons and enhanced green fluorescent protein-expressing transplanted NPCs.

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