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Temporal recording of mammalian development and precancer.

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Peer-reviewed

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https://www.repository.cam.ac.uk/handle/1810/375662

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Type

Article

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Authors

Islam, Mirazul  ORCID logo  https://orcid.org/0000-0003-4959-739X
Yang, Yilin  ORCID logo  https://orcid.org/0009-0000-9869-4044
Simmons, Alan J  ORCID logo  https://orcid.org/0000-0002-3412-5819
Musale, Krushna Pavan  ORCID logo  https://orcid.org/0000-0002-7856-8224

Abstract

Temporal ordering of cellular events offers fundamental insights into biological phenomena. Although this is traditionally achieved through continuous direct observations1,2, an alternative solution leverages irreversible genetic changes, such as naturally occurring mutations, to create indelible marks that enables retrospective temporal ordering3-5. Using a multipurpose, single-cell CRISPR platform, we developed a molecular clock approach to record the timing of cellular events and clonality in vivo, with incorporation of cell state and lineage information. Using this approach, we uncovered precise timing of tissue-specific cell expansion during mouse embryonic development, unconventional developmental relationships between cell types and new epithelial progenitor states by their unique genetic histories. Analysis of mouse adenomas, coupled to multiomic and single-cell profiling of human precancers, with clonal analysis of 418 human polyps, demonstrated the occurrence of polyclonal initiation in 15-30% of colonic precancers, showing their origins from multiple normal founders. Our study presents a multimodal framework that lays the foundation for in vivo recording, integrating synthetic or natural indelible genetic changes with single-cell analyses, to explore the origins and timing of development and tumorigenesis in mammalian systems.

Description

Acknowledgements: This publication is part of the HTAN consortium paper package. We thank the study participants and funding support by HTAN (nos. U2CCA233291 to R.J.C., K.S.L. and M.J.S.), TBEL (U54CA274367 to R.J.C., K.S.L. and M.J.S., R35CA197570 and P50CA236733 to R.J.C., R01DK103831 to K.S.L., K07CA122451 to M.J.S. and R01HG012357 to R.K.) and the Stanley Cohen Innovation Fund (to K.S.L). H.Z. is supported by SRG/2020/001333. We thank members of the Lau and Coffey laboratories (in particular, M. E. Bechard and S. E. Glass) for technical and editorial assistance. Cores used in this study included Survey and Biospecimen Shared Resource, TPSR (no. P30DK058404), VANTAGE (no. P30CA068485) and REDCap (no. UL1TR000445). 1cellbio and RAN biotechnologies helped in the synthesis of custom hydrogel beads. We also thank A. Hasty and A. Jones (VANTAGE) for their assistance. Vanderbilt University has submitted a US patent application for NSC–seq, with M.I., R.J.C. and K.S.L. listed as inventors. We apologize in advance to those we have failed to acknowledge due to space constraints. R.J.C. acknowledges the generous support of the Nicholas Tierney GI Cancer Memorial Fund.

Keywords

Animals, Female, Humans, Male, Mice, Adenoma, Carcinogenesis, Cell Lineage, Clone Cells, Colonic Neoplasms, CRISPR-Cas Systems, Embryonic Development, Organ Specificity, Precancerous Conditions, Single-Cell Analysis, Time Factors, Multiomics, Polyps

Journal Title

Nature

Conference Name

Journal ISSN

0028-0836
1476-4687

Volume Title

634

Publisher

Springer Nature

Publisher DOI

https://doi.org/10.1038/s41586-024-07954-4

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Except where otherwised noted, this item's license is described as http://creativecommons.org/licenses/by-nc-nd/4.0/

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