Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens

In three-dimensional light microscopy, the heterogeneity of the optical density in a specimen ultimately limits the achievable penetration depth and hence the three-dimensional resolution. The most direct approach to reduce aberrations, improve the contrast and achieve an optimal resolution is to mi...

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Autores principales: Hötte, Katharina, Koch, Michael, Hof, Lotta, Tuppi, Marcel, Moreth, Till, Verstegen, Monique M. A., van der Laan, Luc J. W., Stelzer, Ernst H. K., Pampaloni, Francesco
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Nature Publishing Group UK 2019
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Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6872575/
https://www.ncbi.nlm.nih.gov/pubmed/31754183
http://dx.doi.org/10.1038/s41598-019-53380-2
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author Hötte, Katharina
Koch, Michael
Hof, Lotta
Tuppi, Marcel
Moreth, Till
Verstegen, Monique M. A.
van der Laan, Luc J. W.
Stelzer, Ernst H. K.
Pampaloni, Francesco
author_facet Hötte, Katharina
Koch, Michael
Hof, Lotta
Tuppi, Marcel
Moreth, Till
Verstegen, Monique M. A.
van der Laan, Luc J. W.
Stelzer, Ernst H. K.
Pampaloni, Francesco
author_sort Hötte, Katharina
collection PubMed
description In three-dimensional light microscopy, the heterogeneity of the optical density in a specimen ultimately limits the achievable penetration depth and hence the three-dimensional resolution. The most direct approach to reduce aberrations, improve the contrast and achieve an optimal resolution is to minimise the impact of changes of the refractive index along an optical path. Many implementations of light sheet fluorescence microscopy operate with a large chamber filled with an aqueous immersion medium and a further inner container with the specimen embedded in a possibly entirely different non-aqueous medium. In order to minimise the impact of the latter on the optical quality of the images, we use multi-facetted cuvettes fabricated from vacuum-formed ultra-thin fluorocarbon (FEP) foils. The ultra-thin FEP-foil cuvettes have a wall thickness of about 10–12 µm. They are impermeable to liquids, but not to gases, inert, durable, mechanically stable and flexible. Importantly, the usually fragile specimen can remain in the same cuvette from seeding to fixation, clearing and observation, without the need to remove or remount it during any of these steps. We confirm the improved imaging performance of ultra-thin FEP-foil cuvettes with excellent quality images of whole organs such us mouse oocytes, of thick tissue sections from mouse brain and kidney as well as of dense pancreas and liver organoid clusters. Our ultra-thin FEP-foil cuvettes outperform many other sample-mounting techniques in terms of a full separation of the specimen from the immersion medium, compatibility with aqueous and organic clearing media, quick specimen mounting without hydrogel embedding and their applicability for multiple-view imaging and automated image segmentation. Additionally, we show that ultra-thin FEP foil cuvettes are suitable for seeding and growing organoids over a time period of at least ten days. The new cuvettes allow the fixation and staining of specimens inside the holder, preserving the delicate morphology of e.g. fragile, mono-layered three-dimensional organoids.
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spelling pubmed-68725752019-12-04 Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens Hötte, Katharina Koch, Michael Hof, Lotta Tuppi, Marcel Moreth, Till Verstegen, Monique M. A. van der Laan, Luc J. W. Stelzer, Ernst H. K. Pampaloni, Francesco Sci Rep Article In three-dimensional light microscopy, the heterogeneity of the optical density in a specimen ultimately limits the achievable penetration depth and hence the three-dimensional resolution. The most direct approach to reduce aberrations, improve the contrast and achieve an optimal resolution is to minimise the impact of changes of the refractive index along an optical path. Many implementations of light sheet fluorescence microscopy operate with a large chamber filled with an aqueous immersion medium and a further inner container with the specimen embedded in a possibly entirely different non-aqueous medium. In order to minimise the impact of the latter on the optical quality of the images, we use multi-facetted cuvettes fabricated from vacuum-formed ultra-thin fluorocarbon (FEP) foils. The ultra-thin FEP-foil cuvettes have a wall thickness of about 10–12 µm. They are impermeable to liquids, but not to gases, inert, durable, mechanically stable and flexible. Importantly, the usually fragile specimen can remain in the same cuvette from seeding to fixation, clearing and observation, without the need to remove or remount it during any of these steps. We confirm the improved imaging performance of ultra-thin FEP-foil cuvettes with excellent quality images of whole organs such us mouse oocytes, of thick tissue sections from mouse brain and kidney as well as of dense pancreas and liver organoid clusters. Our ultra-thin FEP-foil cuvettes outperform many other sample-mounting techniques in terms of a full separation of the specimen from the immersion medium, compatibility with aqueous and organic clearing media, quick specimen mounting without hydrogel embedding and their applicability for multiple-view imaging and automated image segmentation. Additionally, we show that ultra-thin FEP foil cuvettes are suitable for seeding and growing organoids over a time period of at least ten days. The new cuvettes allow the fixation and staining of specimens inside the holder, preserving the delicate morphology of e.g. fragile, mono-layered three-dimensional organoids. Nature Publishing Group UK 2019-11-21 /pmc/articles/PMC6872575/ /pubmed/31754183 http://dx.doi.org/10.1038/s41598-019-53380-2 Text en © The Author(s) 2019 Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The images or other third party material in this article are included in the article’s Creative Commons license, unless indicated otherwise in a credit line to the material. If material is not included in the article’s Creative Commons license and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this license, visit http://creativecommons.org/licenses/by/4.0/.
spellingShingle Article
Hötte, Katharina
Koch, Michael
Hof, Lotta
Tuppi, Marcel
Moreth, Till
Verstegen, Monique M. A.
van der Laan, Luc J. W.
Stelzer, Ernst H. K.
Pampaloni, Francesco
Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title_full Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title_fullStr Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title_full_unstemmed Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title_short Ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
title_sort ultra-thin fluorocarbon foils optimise multiscale imaging of three-dimensional native and optically cleared specimens
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6872575/
https://www.ncbi.nlm.nih.gov/pubmed/31754183
http://dx.doi.org/10.1038/s41598-019-53380-2
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