Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging

Two-photon excitation microscopy is one of the key techniques used to observe three-dimensional (3-D) structures in biological samples. We utilized a visible-wavelength laser beam for two-photon excitation in a multifocus confocal scanning system to improve the spatial resolution and image contrast...

Descripción completa

Detalles Bibliográficos
Autores principales: Oketani, Ryosuke, Suda, Haruka, Uegaki, Kumiko, Kubo, Toshiki, Matsuda, Tomoki, Yamanaka, Masahito, Arai, Yoshiyuki, Smith, Nicholas I., Nagai, Takeharu, Fujita, Katsumasa
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Society of Photo-Optical Instrumentation Engineers 2019
Materias:
Special Section Celebrating Thirty Years of Multiphoton Microscopy in the Biomedical Sciences
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7008499/
https://www.ncbi.nlm.nih.gov/pubmed/31691550
http://dx.doi.org/10.1117/1.JBO.25.1.014502
_version_ 1783495479764451328
author Oketani, Ryosuke
Suda, Haruka
Uegaki, Kumiko
Kubo, Toshiki
Matsuda, Tomoki
Yamanaka, Masahito
Arai, Yoshiyuki
Smith, Nicholas I.
Nagai, Takeharu
Fujita, Katsumasa
author_facet Oketani, Ryosuke
Suda, Haruka
Uegaki, Kumiko
Kubo, Toshiki
Matsuda, Tomoki
Yamanaka, Masahito
Arai, Yoshiyuki
Smith, Nicholas I.
Nagai, Takeharu
Fujita, Katsumasa
author_sort Oketani, Ryosuke
collection PubMed
description Two-photon excitation microscopy is one of the key techniques used to observe three-dimensional (3-D) structures in biological samples. We utilized a visible-wavelength laser beam for two-photon excitation in a multifocus confocal scanning system to improve the spatial resolution and image contrast in 3-D live-cell imaging. Experimental and numerical analyses revealed that the axial resolution has improved for a wide range of pinhole sizes used for confocal detection. We observed the 3-D movements of the Golgi bodies in living HeLa cells with an imaging speed of 2 s per volume. We also confirmed that the time-lapse observation up to 8 min did not cause significant cell damage in two-photon excitation experiments using wavelengths in the visible light range. These results demonstrate that multifocus, two-photon excitation microscopy with the use of a visible wavelength can constitute a simple technique for 3-D visualization of living cells with high spatial resolution and image contrast.
format Online
Article
Text
id pubmed-7008499
institution National Center for Biotechnology Information
language English
publishDate 2019
publisher Society of Photo-Optical Instrumentation Engineers
record_format MEDLINE/PubMed
spelling pubmed-70084992020-02-14 Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging Oketani, Ryosuke Suda, Haruka Uegaki, Kumiko Kubo, Toshiki Matsuda, Tomoki Yamanaka, Masahito Arai, Yoshiyuki Smith, Nicholas I. Nagai, Takeharu Fujita, Katsumasa J Biomed Opt Special Section Celebrating Thirty Years of Multiphoton Microscopy in the Biomedical Sciences Two-photon excitation microscopy is one of the key techniques used to observe three-dimensional (3-D) structures in biological samples. We utilized a visible-wavelength laser beam for two-photon excitation in a multifocus confocal scanning system to improve the spatial resolution and image contrast in 3-D live-cell imaging. Experimental and numerical analyses revealed that the axial resolution has improved for a wide range of pinhole sizes used for confocal detection. We observed the 3-D movements of the Golgi bodies in living HeLa cells with an imaging speed of 2 s per volume. We also confirmed that the time-lapse observation up to 8 min did not cause significant cell damage in two-photon excitation experiments using wavelengths in the visible light range. These results demonstrate that multifocus, two-photon excitation microscopy with the use of a visible wavelength can constitute a simple technique for 3-D visualization of living cells with high spatial resolution and image contrast. Society of Photo-Optical Instrumentation Engineers 2019-11-05 2020-01 /pmc/articles/PMC7008499/ /pubmed/31691550 http://dx.doi.org/10.1117/1.JBO.25.1.014502 Text en © 2020 The Authors https://creativecommons.org/licenses/by/4.0/ Published by SPIE under a Creative Commons Attribution 4.0 Unported License. Distribution or reproduction of this work in whole or in part requires full attribution of the original publication, including its DOI.
spellingShingle Special Section Celebrating Thirty Years of Multiphoton Microscopy in the Biomedical Sciences
Oketani, Ryosuke
Suda, Haruka
Uegaki, Kumiko
Kubo, Toshiki
Matsuda, Tomoki
Yamanaka, Masahito
Arai, Yoshiyuki
Smith, Nicholas I.
Nagai, Takeharu
Fujita, Katsumasa
Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title_full Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title_fullStr Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title_full_unstemmed Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title_short Visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
title_sort visible-wavelength two-photon excitation microscopy with multifocus scanning for volumetric live-cell imaging
topic Special Section Celebrating Thirty Years of Multiphoton Microscopy in the Biomedical Sciences
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7008499/
https://www.ncbi.nlm.nih.gov/pubmed/31691550
http://dx.doi.org/10.1117/1.JBO.25.1.014502
work_keys_str_mv AT oketaniryosuke visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT sudaharuka visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT uegakikumiko visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT kubotoshiki visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT matsudatomoki visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT yamanakamasahito visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT araiyoshiyuki visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT smithnicholasi visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT nagaitakeharu visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging
AT fujitakatsumasa visiblewavelengthtwophotonexcitationmicroscopywithmultifocusscanningforvolumetriclivecellimaging

Ejemplares similares