4.7 Article

Single Nuclei Analyses Reveal Transcriptional Profiles and Marker Genes for Diverse Supraspinal Populations

Journal

JOURNAL OF NEUROSCIENCE
Volume 42, Issue 47, Pages 8780-8794

Publisher

SOC NEUROSCIENCE
DOI: 10.1523/JNEUROSCI.1197-22.2022

Keywords

AAV2-retro; growth factor receptor; guidance receptor; scRNA-seq; supraspinal neuron; transcription factor

Categories

Funding

  1. National Institute of Neurological Disorders and Stroke
  2. Bryon Riesch Paralysis Foundation
  3. Miami Project to Cure Paralysis
  4. Buoniconti Fund

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This study analyzed neurons projecting from the brain to the spinal cord in mice, identifying 14 transcriptionally distinct cell types and marker genes. The findings provide insights into the molecular characteristics and physiological functions of supraspinal cell populations.
The mammalian brain contains numerous neurons distributed across forebrain, midbrain, and hindbrain that project axons to the lower spinal cord and work in concert to control movement and achieve homeostasis. Extensive work has mapped the anatomic location of supraspinal cell types and continues to establish specific physiological functions. The patterns of gene expression that typify and distinguish these disparate populations, however, are mostly unknown. Here, using adult mice of mixed sex, we combined retrograde labeling of supraspinal cell nuclei with fluorescence-activated nuclei sorting and single -nuclei RNA sequencing analyses to transcriptionally profile neurons that project axons from the brain to lumbar spinal cord. We identified 14 transcriptionally distinct cell types and used a combination of established and newly identified marker genes to assign an anatomic location to each. To validate the putative marker genes, we visualized selected transcripts and con-firmed selective expression within lumbar-projecting neurons in discrete supraspinal regions. Finally, we illustrate the poten-tial utility of these data by examining the expression of transcription factors that distinguish different supraspinal cell types and by surveying the expression of receptors for growth and guidance cues that may be present in the spinal cord. Collectively, these data establish transcriptional differences between anatomically defined supraspinal populations, identify a new set of marker genes of use in future experiments, and provide insight into potential differences in cellular and physiolog-ical activity across the supraspinal connectome.

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