Two-photon excitation of channelrhodopsin-2 at saturation

Abstract: We demonstrate that channelrhodopsin-2 (CR), a light-gated ion channel that is conventionally activated by using visible-light excitation, can also be activated by using IR two-photon excitation (TPE). An empirical estimate of CR's two-photon absorption crosssection at λ = 920 nm is presented, with a value (260 ± 20 GM) indicating that TPE stimulation of CR photocurrents is not typically limited by intrinsic molecular excitability [1 GM = 10 −50 (cm 4 s)/ photon]. By using direct physiological measurements of … Show more

“…Because MAGs can be used for controlling neuron depolarization when tethered to an engineered ion channel (e.g., LiGluR), we note that the 2P absorption cross-sections are smaller than that of Channelrhodopsin2 (230-260 GM) (12,39). Although it can be difficult to compare σ 2 values measured by different methods (16,17), Yamaguchi and Tahara reported a comparable σ 2 of 230 GM for all-trans retinal in solution determined by the same 2P spectrophotometry technique used here (39).…”

“…However, L-MAG0 460 offer some flexibility in 2P excitation compared with opsins because of their relatively slow off-kinetics (52,53). Two-photon stimulation of opsins with fast off-kinetics has required creative use of scanning algorithms (12) or scanless imaging methods (54) to achieve sufficient summation. Opsins that are specifically engineered to have slower off-kinetics can be excited by 2P laser scanning (11), although larger currents still are obtained by 2P-DH (34).…”

“…Brightness, defined for fluorophores as the product of absorption cross-section and fluorescence quantum yield, gives the experimenter an objective metric to assess fluorescent reporters and identify appropriate optical parameters, such as the optimal excitation wavelength and range of light intensities (18). By comparison, relatively little information is available on the 2P properties of optogenetic and photopharmacological tools (12,14). Wider adoption of 2P optical manipulations should follow from quantitative characterization of 2P brightness for optogenetic and photopharmacological reagents.…”

“…In particular, the inherent spatial confinement of 2P absorption is critical for optical manipulation of individual cells (10) in the intact mammalian brain, where it is difficult to control the spatial extent of gene expression or confine soluble reagents. However, 2P-excited optogenetics is not yet as widespread in adoption as 2PM, being widely perceived to require sophisticated optical techniques (11)(12)(13) or reagent concentrations that compromise pharmacological specificity (2,14).…”

Two-photon brightness of azobenzene photoswitches designed for glutamate receptor optogenetics

“…Because MAGs can be used for controlling neuron depolarization when tethered to an engineered ion channel (e.g., LiGluR), we note that the 2P absorption cross-sections are smaller than that of Channelrhodopsin2 (230-260 GM) (12,39). Although it can be difficult to compare σ 2 values measured by different methods (16,17), Yamaguchi and Tahara reported a comparable σ 2 of 230 GM for all-trans retinal in solution determined by the same 2P spectrophotometry technique used here (39).…”

“…However, L-MAG0 460 offer some flexibility in 2P excitation compared with opsins because of their relatively slow off-kinetics (52,53). Two-photon stimulation of opsins with fast off-kinetics has required creative use of scanning algorithms (12) or scanless imaging methods (54) to achieve sufficient summation. Opsins that are specifically engineered to have slower off-kinetics can be excited by 2P laser scanning (11), although larger currents still are obtained by 2P-DH (34).…”

“…Brightness, defined for fluorophores as the product of absorption cross-section and fluorescence quantum yield, gives the experimenter an objective metric to assess fluorescent reporters and identify appropriate optical parameters, such as the optimal excitation wavelength and range of light intensities (18). By comparison, relatively little information is available on the 2P properties of optogenetic and photopharmacological tools (12,14). Wider adoption of 2P optical manipulations should follow from quantitative characterization of 2P brightness for optogenetic and photopharmacological reagents.…”

“…In particular, the inherent spatial confinement of 2P absorption is critical for optical manipulation of individual cells (10) in the intact mammalian brain, where it is difficult to control the spatial extent of gene expression or confine soluble reagents. However, 2P-excited optogenetics is not yet as widespread in adoption as 2PM, being widely perceived to require sophisticated optical techniques (11)(12)(13) or reagent concentrations that compromise pharmacological specificity (2,14).…”

Two-photon brightness of azobenzene photoswitches designed for glutamate receptor optogenetics

“…Single molecule fluorescence in biological systems requires highly localized optical excitation. 8,9 Several techniques have been used to reduce the excitation volume, including laser focusing, 10,11 two photon excitation, 12,13 4Pi, 14 image interference and incoherent interference illumination microscopy (I5M), 15 and near field excitation. 16,17 However, most of these methods involve complex and bulky optical systems.…”

ZnO nanotube waveguide arrays on graphene films for local optical excitation on biological cells

Two‐Photon Excitation Microscopy for the Study of Living Cells and Tissues