Literature DB >> 34462592

High-speed, cortex-wide volumetric recording of neuroactivity at cellular resolution using light beads microscopy.

Jeffrey Demas1,2, Jason Manley1,2, Frank Tejera1, Kevin Barber1, Hyewon Kim1, Francisca Martínez Traub1, Brandon Chen1, Alipasha Vaziri3,4.   

Abstract

Two-photon microscopy has enabled high-resolution imaging of neuroactivity at depth within scattering brain tissue. However, its various realizations have not overcome the tradeoffs between speed and spatiotemporal sampling that would be necessary to enable mesoscale volumetric recording of neuroactivity at cellular resolution and speed compatible with resolving calcium transients. Here, we introduce light beads microscopy (LBM), a scalable and spatiotemporally optimal acquisition approach limited only by fluorescence lifetime, where a set of axially separated and temporally distinct foci record the entire axial imaging range near-simultaneously, enabling volumetric recording at 1.41 × 108 voxels per second. Using LBM, we demonstrate mesoscopic and volumetric imaging at multiple scales in the mouse cortex, including cellular-resolution recordings within ~3 × 5 × 0.5 mm volumes containing >200,000 neurons at ~5 Hz and recordings of populations of ~1 million neurons within ~5.4 × 6 × 0.5 mm volumes at ~2 Hz, as well as higher speed (9.6 Hz) subcellular-resolution volumetric recordings. LBM provides an opportunity for discovering the neurocomputations underlying cortex-wide encoding and processing of information in the mammalian brain.
© 2021. The Author(s), under exclusive licence to Springer Nature America, Inc.

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Year:  2021        PMID: 34462592      PMCID: PMC8958902          DOI: 10.1038/s41592-021-01239-8

Source DB:  PubMed          Journal:  Nat Methods        ISSN: 1548-7091            Impact factor:   28.547


  46 in total

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  27 in total

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Review 9.  Volumetric Imaging of Neural Activity by Light Field Microscopy.

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10.  On the prediction of neuronal microscale topology descriptors based on mesoscale recordings.

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