Two-photon optogenetic toolbox for fast inhibition, excitation and bistable modulation

Rohit Prakash; Ofer Yizhar; Benjamin Grewe; Charu Ramakrishnan; Nancy Wang; Inbal Goshen; Adam M. Packer; Darcy S. Peterka; Rafael Yuste; Mark J. Schnitzer; Karl Deisseroth

doi:10.1038/nmeth.2215

Two-photon optogenetic toolbox for fast inhibition, excitation and bistable modulation

Rohit Prakash, Ofer Yizhar, Benjamin Grewe, Charu Ramakrishnan, Nancy Wang, Inbal Goshen, Adam M. Packer, Darcy S. Peterka, Rafael Yuste, Mark J. Schnitzer, Karl Deisseroth

Research output: Contribution to journal › Article › peer-review

Abstract

Optogenetics with microbial opsin genes has enabled high-speed control of genetically specified cell populations in intact tissue. However, it remains a challenge to independently control subsets of cells within the genetically targeted population. Although spatially precise excitation of target molecules can be achieved using two-photon laser-scanning microscopy (TPLSM) hardware, the integration of two-photon excitation with optogenetics has thus far required specialized equipment or scanning and has not yet been widely adopted. Here we take a complementary approach, developing opsins with custom kinetic, expression and spectral properties uniquely suited to scan times typical of the raster approach that is ubiquitous in TPLSM laboratories. We use a range of culture, slice and mammalian in vivo preparations to demonstrate the versatility of this toolbox, and we quantitatively map parameter space for fast excitation, inhibition and bistable control. Together these advances may help enable broad adoption of integrated optogenetic and TPLSM technologies across experimental fields and systems.

Original language	English
Pages (from-to)	1171-1179
Number of pages	9
Journal	Nature Methods
Volume	9
Issue number	12
DOIs	https://doi.org/10.1038/nmeth.2215
State	Published - Dec 2012
Externally published	Yes

All Science Journal Classification (ASJC) codes

Biotechnology
Biochemistry
Molecular Biology
Cell Biology

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title = "Two-photon optogenetic toolbox for fast inhibition, excitation and bistable modulation",

abstract = "Optogenetics with microbial opsin genes has enabled high-speed control of genetically specified cell populations in intact tissue. However, it remains a challenge to independently control subsets of cells within the genetically targeted population. Although spatially precise excitation of target molecules can be achieved using two-photon laser-scanning microscopy (TPLSM) hardware, the integration of two-photon excitation with optogenetics has thus far required specialized equipment or scanning and has not yet been widely adopted. Here we take a complementary approach, developing opsins with custom kinetic, expression and spectral properties uniquely suited to scan times typical of the raster approach that is ubiquitous in TPLSM laboratories. We use a range of culture, slice and mammalian in vivo preparations to demonstrate the versatility of this toolbox, and we quantitatively map parameter space for fast excitation, inhibition and bistable control. Together these advances may help enable broad adoption of integrated optogenetic and TPLSM technologies across experimental fields and systems.",

author = "Rohit Prakash and Ofer Yizhar and Benjamin Grewe and Charu Ramakrishnan and Nancy Wang and Inbal Goshen and Packer, \{Adam M.\} and Peterka, \{Darcy S.\} and Rafael Yuste and Schnitzer, \{Mark J.\} and Karl Deisseroth",

note = "Funding Information: We thank R. Pashaie and the Deisseroth laboratory members for helpful discussions. We thank Prairie Technologies (T. Keifer, M. Szulczewsk and A. Statz) for discussions and work with the two-photon microscope. R.P. is supported by the US National Institute of Mental Health (F30 MH095468). K.D. is supported by the US National Institutes of Health, the Gatsby Foundation and the Defense Advanced Research Program Agency REPAIR Program.",

year = "2012",

month = dec,

doi = "10.1038/nmeth.2215",

language = "الإنجليزيّة",

volume = "9",

pages = "1171--1179",

journal = "Nature Methods",

issn = "1548-7091",

publisher = "Nature Research",

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TY - JOUR

T1 - Two-photon optogenetic toolbox for fast inhibition, excitation and bistable modulation

AU - Prakash, Rohit

AU - Yizhar, Ofer

AU - Grewe, Benjamin

AU - Ramakrishnan, Charu

AU - Wang, Nancy

AU - Goshen, Inbal

AU - Packer, Adam M.

AU - Peterka, Darcy S.

AU - Yuste, Rafael

AU - Schnitzer, Mark J.

AU - Deisseroth, Karl

N1 - Funding Information: We thank R. Pashaie and the Deisseroth laboratory members for helpful discussions. We thank Prairie Technologies (T. Keifer, M. Szulczewsk and A. Statz) for discussions and work with the two-photon microscope. R.P. is supported by the US National Institute of Mental Health (F30 MH095468). K.D. is supported by the US National Institutes of Health, the Gatsby Foundation and the Defense Advanced Research Program Agency REPAIR Program.

PY - 2012/12

Y1 - 2012/12

N2 - Optogenetics with microbial opsin genes has enabled high-speed control of genetically specified cell populations in intact tissue. However, it remains a challenge to independently control subsets of cells within the genetically targeted population. Although spatially precise excitation of target molecules can be achieved using two-photon laser-scanning microscopy (TPLSM) hardware, the integration of two-photon excitation with optogenetics has thus far required specialized equipment or scanning and has not yet been widely adopted. Here we take a complementary approach, developing opsins with custom kinetic, expression and spectral properties uniquely suited to scan times typical of the raster approach that is ubiquitous in TPLSM laboratories. We use a range of culture, slice and mammalian in vivo preparations to demonstrate the versatility of this toolbox, and we quantitatively map parameter space for fast excitation, inhibition and bistable control. Together these advances may help enable broad adoption of integrated optogenetic and TPLSM technologies across experimental fields and systems.

AB - Optogenetics with microbial opsin genes has enabled high-speed control of genetically specified cell populations in intact tissue. However, it remains a challenge to independently control subsets of cells within the genetically targeted population. Although spatially precise excitation of target molecules can be achieved using two-photon laser-scanning microscopy (TPLSM) hardware, the integration of two-photon excitation with optogenetics has thus far required specialized equipment or scanning and has not yet been widely adopted. Here we take a complementary approach, developing opsins with custom kinetic, expression and spectral properties uniquely suited to scan times typical of the raster approach that is ubiquitous in TPLSM laboratories. We use a range of culture, slice and mammalian in vivo preparations to demonstrate the versatility of this toolbox, and we quantitatively map parameter space for fast excitation, inhibition and bistable control. Together these advances may help enable broad adoption of integrated optogenetic and TPLSM technologies across experimental fields and systems.

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U2 - 10.1038/nmeth.2215

DO - 10.1038/nmeth.2215

M3 - مقالة

C2 - 23169303

SN - 1548-7091

VL - 9

SP - 1171

EP - 1179

JO - Nature Methods

JF - Nature Methods

IS - 12

ER -

Two-photon optogenetic toolbox for fast inhibition, excitation and bistable modulation

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