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Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning

Due to the overlapping emission spectra of fluorophores, fluorescence microscopy images often have bleed-through problems, leading to a false positive detection. This problem is almost unavoidable when the samples are labeled with three or more fluorophores, and the situation is complicated even fur...

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Autores principales: McRae, Tristan D., Oleksyn, David, Miller, Jim, Gao, Yu-Rong
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6886781/
https://www.ncbi.nlm.nih.gov/pubmed/31790435
http://dx.doi.org/10.1371/journal.pone.0225410
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author McRae, Tristan D.
Oleksyn, David
Miller, Jim
Gao, Yu-Rong
author_facet McRae, Tristan D.
Oleksyn, David
Miller, Jim
Gao, Yu-Rong
author_sort McRae, Tristan D.
collection PubMed
description Due to the overlapping emission spectra of fluorophores, fluorescence microscopy images often have bleed-through problems, leading to a false positive detection. This problem is almost unavoidable when the samples are labeled with three or more fluorophores, and the situation is complicated even further when imaged under a multiphoton microscope. Several methods have been developed and commonly used by biologists for fluorescence microscopy spectral unmixing, such as linear unmixing, non-negative matrix factorization, deconvolution, and principal component analysis. However, they either require pre-knowledge of emission spectra or restrict the number of fluorophores to be the same as detection channels, which highly limits the real-world applications of those spectral unmixing methods. In this paper, we developed a robust and flexible spectral unmixing method: Learning Unsupervised Means of Spectra (LUMoS), which uses an unsupervised machine learning clustering method to learn individual fluorophores’ spectral signatures from mixed images, and blindly separate channels without restrictions on the number of fluorophores that can be imaged. This method highly expands the hardware capability of two-photon microscopy to simultaneously image more fluorophores than is possible with instrumentation alone. Experimental and simulated results demonstrated the robustness of LUMoS in multi-channel separations of two-photon microscopy images. We also extended the application of this method to background/autofluorescence removal and colocalization analysis. Lastly, we integrated this tool into ImageJ to offer an easy to use spectral unmixing tool for fluorescence imaging. LUMoS allows us to gain a higher spectral resolution and obtain a cleaner image without the need to upgrade the imaging hardware capabilities.
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spelling pubmed-68867812019-12-13 Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning McRae, Tristan D. Oleksyn, David Miller, Jim Gao, Yu-Rong PLoS One Research Article Due to the overlapping emission spectra of fluorophores, fluorescence microscopy images often have bleed-through problems, leading to a false positive detection. This problem is almost unavoidable when the samples are labeled with three or more fluorophores, and the situation is complicated even further when imaged under a multiphoton microscope. Several methods have been developed and commonly used by biologists for fluorescence microscopy spectral unmixing, such as linear unmixing, non-negative matrix factorization, deconvolution, and principal component analysis. However, they either require pre-knowledge of emission spectra or restrict the number of fluorophores to be the same as detection channels, which highly limits the real-world applications of those spectral unmixing methods. In this paper, we developed a robust and flexible spectral unmixing method: Learning Unsupervised Means of Spectra (LUMoS), which uses an unsupervised machine learning clustering method to learn individual fluorophores’ spectral signatures from mixed images, and blindly separate channels without restrictions on the number of fluorophores that can be imaged. This method highly expands the hardware capability of two-photon microscopy to simultaneously image more fluorophores than is possible with instrumentation alone. Experimental and simulated results demonstrated the robustness of LUMoS in multi-channel separations of two-photon microscopy images. We also extended the application of this method to background/autofluorescence removal and colocalization analysis. Lastly, we integrated this tool into ImageJ to offer an easy to use spectral unmixing tool for fluorescence imaging. LUMoS allows us to gain a higher spectral resolution and obtain a cleaner image without the need to upgrade the imaging hardware capabilities. Public Library of Science 2019-12-02 /pmc/articles/PMC6886781/ /pubmed/31790435 http://dx.doi.org/10.1371/journal.pone.0225410 Text en © 2019 McRae et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
McRae, Tristan D.
Oleksyn, David
Miller, Jim
Gao, Yu-Rong
Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title_full Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title_fullStr Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title_full_unstemmed Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title_short Robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
title_sort robust blind spectral unmixing for fluorescence microscopy using unsupervised learning
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6886781/
https://www.ncbi.nlm.nih.gov/pubmed/31790435
http://dx.doi.org/10.1371/journal.pone.0225410
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