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Unraveling Subcellular Ultrastructure with Cyclically Multiplexed Expansion Microscopy

Abstract:
Despite advances in fluorescence microscopy, spectral overlap and limited resolution hinder the dense mapping of the cellular ultrastructure. To overcome these challenges, we developed Cy-ExM, a high-plex imaging strategy that integrates optimized cryo-fixation for antigen preservation, expansion microscopy, and iterative immunofluorescence labeling. Using oblique plane microscopy, we perform three-dimensional super-resolution imaging of 20 biological targets encompassing the full cellular volume of individual mammalian cells.
Publication status:
Published
Peer review status:
Peer reviewed

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Publisher copy:
10.64898/2026.01.01.697161

Authors

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Role:
Author
ORCID:
0000-0002-7020-0804
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Role:
Author
ORCID:
0000-0002-5513-7106
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Institution:
University of Oxford
Role:
Author
ORCID:
0000-0003-4463-1165
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Role:
Author
ORCID:
0000-0002-2808-4408
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Role:
Author
ORCID:
0000-0001-9666-7923


Publisher:
openRxiv
Journal:
bioRxiv More from this journal
Publication date:
2026-01-02
DOI:
EISSN:
2692-8205


Language:
English
Keywords:
Pubs id:
2409307
Local pid:
pubs:2409307
Source identifiers:
W7117986318
Deposit date:
2026-04-21
ARK identifier:
This ORA record was generated from metadata provided by an external service. It has not been edited by the ORA Team.

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