Three-photon excited fluorescence microscopy enables imaging of blood flow, neural structure and inflammatory response deep into mouse spinal cord in vivo

Author:

Cheng Yu-Ting12,Lett Kawasi M.1,Xu Chris3ORCID,Schaffer Chris B.1ORCID

Affiliation:

1. Nancy E. and Peter C. Meinig School of Biomedical Engineering, Cornell University

2. Department of Neurobiology and Behavior, Cornell University

3. School of Applied and Engineering Physics, Cornell University

Abstract

Nonlinear optical microscopy enables non-invasive imaging in scattering samples with cellular resolution. The spinal cord connects the brain with the periphery and governs fundamental behaviors such as locomotion and somatosensation. Because of dense myelination on the dorsal surface, imaging to the spinal grey matter is challenging, even with two-photon microscopy. Here we show that three-photon excited fluorescence (3PEF) microscopy enables multicolor imaging at depths of up to ~550 μm into the mouse spinal cord, in vivo . We quantified blood flow across vessel types along the spinal vascular network. We then followed the response of neurites and microglia after occlusion of a surface venule, where we observed depth-dependent structural changes in neurites and interactions of perivascular microglia with vessel branches upstream from the clot. This work establishes that 3PEF imaging enables studies of functional dynamics and cell type interactions in the top 550 μm of the murine spinal cord, in vivo .

Publisher

eLife Sciences Publications, Ltd

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