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A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy

We present a new convenient method for quantitative three-dimensionally resolved diffusion measurements based on the photobleaching (FRAP) or photoactivation (FRAPa) of a disk-shaped area by the scanning laser beam of a multiphoton microscope. Contrary to previously reported spot-photobleaching prot...

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Autores principales: Mazza, Davide, Braeckmans, Kevin, Cella, Francesca, Testa, Ilaria, Vercauteren, Dries, Demeester, Jo, De Smedt, Stefaan S., Diaspro, Alberto
Formato: Texto
Lenguaje:English
Publicado: The Biophysical Society 2008
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2547427/
https://www.ncbi.nlm.nih.gov/pubmed/18621824
http://dx.doi.org/10.1529/biophysj.108.133637
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author Mazza, Davide
Braeckmans, Kevin
Cella, Francesca
Testa, Ilaria
Vercauteren, Dries
Demeester, Jo
De Smedt, Stefaan S.
Diaspro, Alberto
author_facet Mazza, Davide
Braeckmans, Kevin
Cella, Francesca
Testa, Ilaria
Vercauteren, Dries
Demeester, Jo
De Smedt, Stefaan S.
Diaspro, Alberto
author_sort Mazza, Davide
collection PubMed
description We present a new convenient method for quantitative three-dimensionally resolved diffusion measurements based on the photobleaching (FRAP) or photoactivation (FRAPa) of a disk-shaped area by the scanning laser beam of a multiphoton microscope. Contrary to previously reported spot-photobleaching protocols, this method has the advantage of full scalability of the size of the photobleached area and thus the range of diffusion coefficients, which can be measured conveniently. The method is compatible with low as well as high numerical aperture objective lenses, allowing us to perform quantitative diffusion measurements in three-dimensional extended samples as well as in very small volumes, such as cell nuclei. Furthermore, by photobleaching/photoactivating a large area, diffusion along the optical axis can be measured separately, which is convenient when studying anisotropic diffusion. First, we show the rigorous mathematical derivation of the model, leading to a closed-form formula describing the fluorescence recovery/redistribution phase. Next, the ability of the multiphoton FRAP method to correctly measure absolute diffusion coefficients is tested thoroughly on many test solutions of FITC-dextrans covering a wide range of diffusion coefficients. The same is done for the FRAPa method on a series of photoactivatable green fluorescent protein solutions with different viscosities. Finally, we apply the method to photoactivatable green fluorescent protein diffusing freely in the nucleus of living NIH-3T3 mouse embryo fibroblasts.
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spelling pubmed-25474272008-10-01 A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy Mazza, Davide Braeckmans, Kevin Cella, Francesca Testa, Ilaria Vercauteren, Dries Demeester, Jo De Smedt, Stefaan S. Diaspro, Alberto Biophys J Spectroscopy, Imaging, Other Techniques We present a new convenient method for quantitative three-dimensionally resolved diffusion measurements based on the photobleaching (FRAP) or photoactivation (FRAPa) of a disk-shaped area by the scanning laser beam of a multiphoton microscope. Contrary to previously reported spot-photobleaching protocols, this method has the advantage of full scalability of the size of the photobleached area and thus the range of diffusion coefficients, which can be measured conveniently. The method is compatible with low as well as high numerical aperture objective lenses, allowing us to perform quantitative diffusion measurements in three-dimensional extended samples as well as in very small volumes, such as cell nuclei. Furthermore, by photobleaching/photoactivating a large area, diffusion along the optical axis can be measured separately, which is convenient when studying anisotropic diffusion. First, we show the rigorous mathematical derivation of the model, leading to a closed-form formula describing the fluorescence recovery/redistribution phase. Next, the ability of the multiphoton FRAP method to correctly measure absolute diffusion coefficients is tested thoroughly on many test solutions of FITC-dextrans covering a wide range of diffusion coefficients. The same is done for the FRAPa method on a series of photoactivatable green fluorescent protein solutions with different viscosities. Finally, we apply the method to photoactivatable green fluorescent protein diffusing freely in the nucleus of living NIH-3T3 mouse embryo fibroblasts. The Biophysical Society 2008-10-01 2008-07-11 /pmc/articles/PMC2547427/ /pubmed/18621824 http://dx.doi.org/10.1529/biophysj.108.133637 Text en Copyright © 2008, Biophysical Society This is an Open Access article distributed under the terms of the Creative Commons-Attribution Noncommercial License (http://www.creativecommons.org/licenses/by-nc/2.0/), which permits unrestricted noncommercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Spectroscopy, Imaging, Other Techniques
Mazza, Davide
Braeckmans, Kevin
Cella, Francesca
Testa, Ilaria
Vercauteren, Dries
Demeester, Jo
De Smedt, Stefaan S.
Diaspro, Alberto
A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title_full A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title_fullStr A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title_full_unstemmed A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title_short A New FRAP/FRAPa Method for Three-Dimensional Diffusion Measurements Based on Multiphoton Excitation Microscopy
title_sort new frap/frapa method for three-dimensional diffusion measurements based on multiphoton excitation microscopy
topic Spectroscopy, Imaging, Other Techniques
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2547427/
https://www.ncbi.nlm.nih.gov/pubmed/18621824
http://dx.doi.org/10.1529/biophysj.108.133637
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