Temporal and spatial topography of cell proliferation in cancer.

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ID: 277021
2022
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Abstract
Proliferation is a fundamental trait of cancer cells, but its properties and spatial organization in tumours are poorly characterized. Here we use highly multiplexed tissue imaging to perform single-cell quantification of cell cycle regulators and then develop robust, multivariate, proliferation metrics. Across diverse cancers, proliferative architecture is organized at two spatial scales: large domains, and smaller niches enriched for specific immune lineages. Some tumour cells express cell cycle regulators in the (canonical) patterns expected of freely growing cells, a phenomenon we refer to as 'cell cycle coherence'. By contrast, the cell cycles of other tumour cell populations are skewed towards specific phases or exhibit non-canonical (incoherent) marker combinations. Coherence varies across space, with changes in oncogene activity and therapeutic intervention, and is associated with aggressive tumour behaviour. Thus, multivariate measures from high-plex tissue images capture clinically significant features of cancer proliferation, a fundamental step in enabling more precise use of anti-cancer therapies.
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gaglia2022temporalnature Use this key to autocite in the manuscript while using SciMatic Manuscript Manager or Thesis Manager
Authors Gaglia, Giorgio;Kabraji, Sheheryar;Rammos, Danae;Dai, Yang;Verma, Ana;Wang, Shu;Mills, Caitlin E;Chung, Mirra;Bergholz, Johann S;Coy, Shannon;Lin, Jia-Ren;Jeselsohn, Rinath;Metzger, Otto;Winer, Eric P;Dillon, Deborah A;Zhao, Jean J;Sorger, Peter K;Santagata, Sandro;
Journal Nature Cell Biology
Year 2022
DOI
10.1038/s41556-022-00860-9
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