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Multispectral live-cell imaging with uncompromised spatiotemporal resolution.

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Peer-reviewed

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https://www.repository.cam.ac.uk/handle/1810/390328

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Supporting information (53.42 MB)
Primary Published version (4.74 MB)
 Published version (65.89 MB)
 Bibliographic metadata (119.25 KB)

Type

Article

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Authors

Kumar, Akaash  ORCID logo  https://orcid.org/0009-0008-0880-1917
McNally, Kerrie E  ORCID logo  https://orcid.org/0000-0003-2376-3003
Zhang, Yuexuan  ORCID logo  https://orcid.org/0009-0003-8672-0745

Abstract

Multispectral imaging is an established method to extend the number of colours usable in fluorescence imaging beyond the typical limit of three or four. However, standard approaches are poorly suited to live-cell imaging owing to the need to separate light into many spectral channels, and unmixing algorithms struggle with low signal-to-noise ratio data. Here we introduce an approach for multispectral imaging in live cells that comprises an iterative spectral unmixing algorithm and eight-channel camera-based image-acquisition hardware. This enables the accurate unmixing of low signal-to-noise ratio datasets captured at video rates, while maintaining diffraction-limited spatial resolution. We use this approach on a commercial spinning-disk confocal microscope and a home-built oblique-plane light-sheet microscope to image one to seven spectrally distinct fluorophore species simultaneously, using both fluorescent protein fusions and small-molecule dyes. We further develop protein-binding proteins (minibinders), labelled with organic fluorophores, and use these in combination with our multispectral imaging approach to study the endosomal trafficking of cell-surface receptors at endogenous levels.

Description

Acknowledgements: J.D.M. thanks A. York and R. Heintzmann for interesting discussions regarding Richardson–Lucy deconvolution and acknowledges support from the Royal Society through a University Research Fellowship (URF/R1/221086 and RF/ERE/221078). K.M. acknowledges support from the Wellcome Trust through a Sir Henry Wellcome Postdoctoral Fellowship (220480/Z/20/Z). E.D. is funded by the Medical Research Council (MRC) (MC_UP_1201/13) and Human Frontier Science Program (Career Development Award CDA00034/2017). J.D.M. and E.D. thank J. Grimmett, T. Darling and I. Clayson for scientific computing infrastructure and support. A.K. and J.D.M. thank the Light Microscopy Facility of the MRC LMB for access to the Zeiss LSM 710 instrument used in this work, and thank the Mechanical and Electronic Workshops of the MRC LMB for their assistance. This work was supported by the MRC, as part of United Kingdom Research and Innovation (also known as UK Research and Innovation) (MC_UP_1201/13). For the purpose of open access, the MRC Laboratory of Molecular Biology has applied a CC BY public copyright licence to any author accepted manuscript version arising.

Keywords

Biological fluorescence, Imaging and sensing, Microscopy

Journal Title

Nat Photonics

Conference Name

Journal ISSN

1749-4885
1749-4893

Volume Title

19

Publisher

Springer Nature

Publisher DOI

https://doi.org/10.1038/s41566-025-01745-7

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Except where otherwised noted, this item's license is described as http://creativecommons.org/licenses/by/4.0/
Sponsorship
RCUK | Medical Research Council (MRC) (MC_UP_1201/13)
Human Frontier Science Program (HFSP) (CDA00034/2017)
Royal Society (URF\R1\221086, RF\ERE\221078)

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