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“Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels
We describe an optical technique using total internal reflection fluorescence (TIRF) microscopy to obtain simultaneous and independent recordings from numerous ion channels via imaging of single-channel Ca(2+) flux. Muscle nicotinic acetylcholine (ACh) receptors made up of αβγδ subunits were express...
| Autores principales: | , |
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| Formato: | Texto |
| Lenguaje: | English |
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The Rockefeller University Press
2005
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| Acceso en línea: | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2266576/ https://www.ncbi.nlm.nih.gov/pubmed/16103278 http://dx.doi.org/10.1085/jgp.200509331 |
| _version_ | 1782151532817416192 |
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| author | Demuro, Angelo Parker, Ian |
| author_facet | Demuro, Angelo Parker, Ian |
| author_sort | Demuro, Angelo |
| collection | PubMed |
| description | We describe an optical technique using total internal reflection fluorescence (TIRF) microscopy to obtain simultaneous and independent recordings from numerous ion channels via imaging of single-channel Ca(2+) flux. Muscle nicotinic acetylcholine (ACh) receptors made up of αβγδ subunits were expressed in Xenopus oocytes, and single channel Ca(2+) fluorescence transients (SCCaFTs) were imaged using a fast (500 fps) electron-multiplied c.c.d. camera with fluo-4 as the indicator. Consistent with their arising through openings of individual nicotinic channels, SCCaFTs were seen only when a nicotinic agonist was present in the bathing solution, were blocked by curare, and increased in frequency as roughly the second power of [ACh]. Their fluorescence amplitudes varied linearly with membrane potential and extrapolated to zero at about +60 mV. The rise and fall times of fluorescence were as fast as 2 ms, providing a kinetic resolution adequate to characterize channel gating kinetics; which showed mean open times of 7.9 and 15.8 ms when activated, respectively, by ACh or suberyldicholine. Simultaneous records were obtained from >400 channels in the imaging field, and we devised a novel “channel chip” representation to depict the resultant large dataset as a single image. The positions of SCCaFTs remained fixed (<100 nm displacement) over tens of seconds, indicating that the nicotinic receptor/channels are anchored in the oocyte membrane; and the spatial distribution of channels appeared random without evidence of clustering. Our results extend single-channel TIRFM imaging to ligand-gated channels that display only partial permeability to Ca(2+), and demonstrate an order-of-magnitude improvement in kinetic resolution. We believe that functional single-channel imaging opens a new approach to ion channel study, having particular advantages over patch-clamp recording in that it is massively parallel, and provides high-resolution spatial information that is inaccessible by electrophysiological techniques. |
| format | Text |
| id | pubmed-2266576 |
| institution | National Center for Biotechnology Information |
| language | English |
| publishDate | 2005 |
| publisher | The Rockefeller University Press |
| record_format | MEDLINE/PubMed |
| spelling | pubmed-22665762008-03-21 “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels Demuro, Angelo Parker, Ian J Gen Physiol Article We describe an optical technique using total internal reflection fluorescence (TIRF) microscopy to obtain simultaneous and independent recordings from numerous ion channels via imaging of single-channel Ca(2+) flux. Muscle nicotinic acetylcholine (ACh) receptors made up of αβγδ subunits were expressed in Xenopus oocytes, and single channel Ca(2+) fluorescence transients (SCCaFTs) were imaged using a fast (500 fps) electron-multiplied c.c.d. camera with fluo-4 as the indicator. Consistent with their arising through openings of individual nicotinic channels, SCCaFTs were seen only when a nicotinic agonist was present in the bathing solution, were blocked by curare, and increased in frequency as roughly the second power of [ACh]. Their fluorescence amplitudes varied linearly with membrane potential and extrapolated to zero at about +60 mV. The rise and fall times of fluorescence were as fast as 2 ms, providing a kinetic resolution adequate to characterize channel gating kinetics; which showed mean open times of 7.9 and 15.8 ms when activated, respectively, by ACh or suberyldicholine. Simultaneous records were obtained from >400 channels in the imaging field, and we devised a novel “channel chip” representation to depict the resultant large dataset as a single image. The positions of SCCaFTs remained fixed (<100 nm displacement) over tens of seconds, indicating that the nicotinic receptor/channels are anchored in the oocyte membrane; and the spatial distribution of channels appeared random without evidence of clustering. Our results extend single-channel TIRFM imaging to ligand-gated channels that display only partial permeability to Ca(2+), and demonstrate an order-of-magnitude improvement in kinetic resolution. We believe that functional single-channel imaging opens a new approach to ion channel study, having particular advantages over patch-clamp recording in that it is massively parallel, and provides high-resolution spatial information that is inaccessible by electrophysiological techniques. The Rockefeller University Press 2005-09 /pmc/articles/PMC2266576/ /pubmed/16103278 http://dx.doi.org/10.1085/jgp.200509331 Text en Copyright © 2005, The Rockefeller University Press This article is distributed under the terms of an Attribution–Noncommercial–Share Alike–No Mirror Sites license for the first six months after the publication date (see http://www.rupress.org/terms). After six months it is available under a Creative Commons License (Attribution–Noncommercial–Share Alike 4.0 Unported license, as described at http://creativecommons.org/licenses/by-nc-sa/4.0/). |
| spellingShingle | Article Demuro, Angelo Parker, Ian “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title | “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title_full | “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title_fullStr | “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title_full_unstemmed | “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title_short | “Optical Patch-clamping”: Single-channel Recording by Imaging Ca(2+) Flux through Individual Muscle Acetylcholine Receptor Channels |
| title_sort | “optical patch-clamping”: single-channel recording by imaging ca(2+) flux through individual muscle acetylcholine receptor channels |
| topic | Article |
| url | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2266576/ https://www.ncbi.nlm.nih.gov/pubmed/16103278 http://dx.doi.org/10.1085/jgp.200509331 |
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