4.4 Article

Mapping brain networks in awake mice using combined optical neural control and fMRI

Journal

JOURNAL OF NEUROPHYSIOLOGY
Volume 105, Issue 3, Pages 1393-1405

Publisher

AMER PHYSIOLOGICAL SOC
DOI: 10.1152/jn.00828.2010

Keywords

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Funding

  1. National Institutes of Health [DP2 OD-002002-01, 1RC1 MH-088182-01, 1RC2 DE-020919-01, 1R01 NS-067199-01, MH-060379, NS-025529]
  2. National Science Foundation (NSF) [0835878, 0848804]
  3. McGovern Institute
  4. Department of Defense
  5. National Alliance for Research on Schizophrenia and Depression
  6. Alfred P. Sloan Foundation
  7. Jerry and Marge Burnett
  8. Society for Neuroscience Research
  9. Massachusetts Institute of Technology Media Laboratory
  10. Benesse Foundation
  11. Wallace H. Coulter Foundation
  12. European Union [201716]
  13. McGovern Institute for Brain Research
  14. Division Of Mathematical Sciences
  15. Direct For Mathematical & Physical Scien [0848804] Funding Source: National Science Foundation

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Desai M, Kahn I, Knoblich U, Bernstein J, Atallah H, Yang A, Kopell N, Buckner RL, Graybiel AM, Moore CI, Boyden ES. Mapping brain networks in awake mice using combined optical neural control and fMRI. J Neurophysiol 105: 1393-1405, 2011. First published December 15, 2010; doi:10.1152/jn.00828.2010. Behaviors and brain disorders involve neural circuits that are widely distributed in the brain. The ability to map the functional connectivity of distributed circuits, and to assess how this connectivity evolves over time, will be facilitated by methods for characterizing the network impact of activating a specific subcircuit, cell type, or projection pathway. We describe here an approach using high-resolution blood oxygenation level-dependent (BOLD) functional MRI (fMRI) of the awake mouse brain-to measure the distributed BOLD response evoked by optical activation of a local, defined cell class expressing the light-gated ion channel channelrhodopsin-2 (ChR2). The utility of this opto-fMRI approach was explored by identifying known cortical and subcortical targets of pyramidal cells of the primary somatosensory cortex (SI) and by analyzing how the set of regions recruited by optogenetically driven SI activity differs between the awake and anesthetized states. Results showed positive BOLD responses in a distributed network that included secondary somatosensory cortex (SII), primary motor cortex (MI), caudoputamen (CP), and contralateral SI (c-SI). Measures in awake compared with anesthetized mice (0.7% isoflurane) showed significantly increased BOLD response in the local region (SI) and indirectly stimulated regions (SII, MI, CP, and c-SI), as well as increased BOLD signal temporal correlations between pairs of regions. These collective results suggest opto-fMRI can provide a controlled means for characterizing the distributed network downstream of a defined cell class in the awake brain. Opto-fMRI may find use in examining causal links between defined circuit elements in diverse behaviors and pathologies.

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