Crystal structure of the channelrhodopsin light-gated cation channel

Kato, Hideaki E.; Zhang, Feng; Yizhar, Ofer; Ramakrishnan, Charu; Nishizawa, Takashi; Hirata, Kunio; Ito, Jin‐ichi; Aita, Yusuke; Tsukazaki, Tomoya; Hayashi, Shigehiko; Hegemann, Peter; Maturana, Andrés D.; Ishitani, Ryuichiro; Deisseroth, Karl; Nureki, Osamu

doi:10.1038/nature10870

Cited by 505 publications

(675 citation statements)

References 46 publications

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“…8). 44 In an FT-IR study on the C1C2 chimera, a water molecule with the O-D stretch at 2378 cm −1 was assigned by its sensitivity to site-directed mutations to a water molecule H-bonded to D292 in the dark state, 45 a residue equivalent to D212 in BR. In the dark state of CaChR1, we estimate the O-H (O-D) frequency of the Hbonded O-H group of a dangling water at 3300 cm −1 (2450 cm −1 ), only slightly upshifted in respect to water W401 of BR and to the above discussed water molecule of the C1C2 chimera.…”

Section: B Active Water Molecules In Cachr1mentioning

confidence: 99%

“…Structural model of CaChR1 derived by homology modeling and build by the SWISS-MODEL server 81 using the C1C2 structure as template (pdb: 3UG9). 44 The gray horizontal lines indicate the membrane part of the channel. The retinal chromophore is located in the middle of the membrane (yellow sticks) and bound via a Schiff base, SB (blue), linkage to the apoprotein.…”

Section: B Active Water Molecules In Cachr1mentioning

confidence: 99%

“…42,43 CrChR2 absorbs maximally at ∼470 nm and shows a photocycle comprising a minimum of four intermediate states: 43 The only ChR whose 3D structure has been resolved to atomic resolution is a chimera construct from CrChR1 and CrChR2 (C1C2). 44 Recently, the first report on active internal water molecules on a ChR was published, performed on the C1C2 chimera. 45 Light-induced FT-IR spectroscopy revealed changes in water O-D vibrations upon illumination at 77 K, i.e., between the closed dark and the early P 1 500 state.…”

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Changes in the hydrogen-bonding strength of internal water molecules and cysteine residues in the conductive state of channelrhodopsin-1

Lórenz-Fonfrı́a

Muders

Schlesinger

et al. 2014

The Journal of Chemical Physics

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Water plays an essential role in the structure and function of proteins, particularly in the less understood class of membrane proteins. As the first of its kind, channelrhodopsin is a light-gated cation channel and paved the way for the new and vibrant field of optogenetics, where nerve cells are activated by light. Still, the molecular mechanism of channelrhodopsin is not understood. Here, we applied time-resolved FT-IR difference spectroscopy to channelrhodopsin-1 from Chlamydomonas augustae. It is shown that the ( −1 ) to moderately strongly (3300 cm −1 ) hydrogen-bonded. Changes in amide A and thiol vibrations report on global and local changes, respectively, associated with the formation of the conductive state. Future studies will aim at assigning the respective cysteine group(s) and at localizing the "dangling" water molecules within the protein, providing a better understanding of their functional relevance in CaChR1.

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Section: B Active Water Molecules In Cachr1mentioning

confidence: 99%

Section: B Active Water Molecules In Cachr1mentioning

confidence: 99%

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confidence: 99%

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Changes in the hydrogen-bonding strength of internal water molecules and cysteine residues in the conductive state of channelrhodopsin-1

Lórenz-Fonfrı́a

Muders

Schlesinger

et al. 2014

The Journal of Chemical Physics

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“…Several successful structure determinations from tiny lipidic cubic phase (LCP) crystals proved the efficiency of this system. In the case described in reference [5], helical data collection using a 1(H) x 10(V) m beam and 0.5 m step was conducted. The total absorbed dose was kept below 5 MGy for each of three MAD datasets by using this concept.…”

Section: User Friendly Gui System For Suggesting Data Collection Stramentioning

confidence: 99%

Achievement of protein micro-crystallography at SPring-8 beamline BL32XU

Hirata

Kawano

Ueno

et al. 2013

J. Phys.: Conf. Ser.

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“…19) In addition, the X-ray crystal structure of C1C2 at 2.3 Å resolution is available, and it provides precise information for three-dimensional architecture of C1C2. 20) Based on the crystal structure, the cavity of the retinal binding pocket does not seem to be large enough to allow incorporation of our synthetic enamine-type Schiff bases, as the retinal binding lysine residue would interfere with the Schiff base. Thus, we constructed two C1C2 mutants to accommodate the larger chromophore: one is C1C2-K296A, in which the lysine at the retinal binding site, K296, was replaced by alanine, and the other is C1C2-K296G, in which lysine 296 was substituted with glycine.…”

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confidence: 99%

Alternative Formation of Red-Shifted Channelrhodopsins: Noncovalent Incorporation with Retinal-Based Enamine-Type Schiff Bases and Mutated Channelopsin

Okitsu

Matsuyama

Yamashita

et al. 2017

CHEMICAL & PHARMACEUTICAL BULLETIN

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Red-shifted channelrhodopsins (ChRs) are attractive for optogenetic tools. We developed a new type of red-shifted ChRs that utilized noncovalent incorporation of retinal and 3,4-dehydroretinal-based enamine-type Schiff bases and mutated channelopsin, C1C2-K296G. These ChRs exhibited absorption maxima that were shifted 10-30 nm toward longer wavelengths than that of C1C2-ChR regenerated with alltrans-retinal.Key words channelrhodopsin; chromophore; red-shift; neuroscience; optogenetics The development of a new method of activating a specific neuron without affecting other cells would greatly benefit neuroscience. Optogenetics-a powerful new technique that enables control of neuronal activity by light-offers a number of advantages over previous electrode-based methods.1-4) In addition, optogenetics appears promising for clarifying neural circuits and understanding the mechanisms of various neurological diseases. 5,6) Channelrhodopsins (ChRs) are members of the rhodopsin family in microbes and consist of the chromophore retinal (1) and a seven-transmembrane helix apoprotein, termed channelopsin (Chop). The amino group of a lysine residue (K296) covalently binds to retinal through a protonated Schiff base (PSB) 7) (Fig. 1a). ChRs function as light-gated cation channels by photoisomerization of the retinal from all-trans to 13-cis forms which results in a conformational change of the protein. Two ChRs, Channelrhodopsin-1 (ChR1) and Channelrhodopsin-2 (ChR2), are now widely used in optogenetics, and they are most sensitive to green and blue light, respectively. 7,8) However, such short-wavelength light cannot deeply penetrate into the neural tissues, and optical fiber implants are often required to target the tissues. A truly noninvasive method for optogenetics requires the development of ChRs that are sensitive to long-wavelength light, and so red-shifted ChRs are sought-after. Toward this purpose, two types of red-shifted ChRs have been made: (i) mutation of amino acids in the vicinity of the retinal pocket, [9][10][11] and (ii) substitution of retinal with other red-shifted chromophores that covalently bind to ChRs through a PSB. [12][13][14] In this Communication, we present new types of redshifted ChRs: red-shifted chromophores 3 and 4, consisting of enamine-conjugated Schiff bases of 1 and 3,4-dehydroretinal (2), that non-covalently binds to chimera ChRs (Fig. 1b). This new red-shifted ChR system would have two benefits: (i) introduction of one or two conjugated double bond(s) into the chromophore would result in absorption of longer wavelength light for a red-shift of the UV-Vis spectrum, and (ii) instead of a covalent bond, formation of the selective chromophorechimera Chop would occur by action of van der Waals forces.Herein, we designed chromophores 3 and 4, which we expected to have red-shifted absorption maxima compared to 1 because the presence of the additional double bonds extended the conjugation of the chromophore.15) The most difficult problems for this study were (i) construction of the enamine-conj...

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Crystal structure of the channelrhodopsin light-gated cation channel

Cited by 505 publications

References 46 publications

Changes in the hydrogen-bonding strength of internal water molecules and cysteine residues in the conductive state of channelrhodopsin-1

Changes in the hydrogen-bonding strength of internal water molecules and cysteine residues in the conductive state of channelrhodopsin-1

Achievement of protein micro-crystallography at SPring-8 beamline BL32XU

Alternative Formation of Red-Shifted Channelrhodopsins: Noncovalent Incorporation with Retinal-Based Enamine-Type Schiff Bases and Mutated Channelopsin

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