Literature DB >> 23702834

Two-way communication with neural networks in vivo using focused light.

Nathan R Wilson1, James Schummers, Caroline A Runyan, Sherry X Yan, Robert E Chen, Yuting Deng, Mriganka Sur.   

Abstract

Neuronal networks process information in a distributed, spatially heterogeneous manner that transcends the layout of electrodes. In contrast, directed and steerable light offers the potential to engage specific cells on demand. We present a unified framework for adapting microscopes to use light for simultaneous in vivo stimulation and recording of cells at fine spatiotemporal resolutions. We use straightforward optics to lock onto networks in vivo, to steer light to activate circuit elements and to simultaneously record from other cells. We then actualize this 'free' augmentation on both an 'open' two-photon microscope and a leading commercial one. By following this protocol, setup of the system takes a few days, and the result is a noninvasive interface to brain dynamics based on directed light, at a network resolution that was not previously possible and which will further improve with the rapid advance in development of optical reporters and effectors. This protocol is for physiologists who are competent with computers and wish to extend hardware and software to interface more fluidly with neuronal networks.

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Year:  2013        PMID: 23702834      PMCID: PMC4118663          DOI: 10.1038/nprot.2013.063

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  52 in total

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4.  Closed-Loop Real-Time Imaging Enables Fully Automated Cell-Targeted Patch-Clamp Neural Recording In Vivo.

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7.  A Platform for Spatiotemporal "Matrix" Stimulation in Brain Networks Reveals Novel Forms of Circuit Plasticity.

Authors:  Nathan R Wilson; Forea L Wang; Naiyan Chen; Sherry X Yan; Amy L Daitch; Bo Shi; Samvaran Sharma; Mriganka Sur
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  7 in total

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