Live cell tagging tracking and isolation for spatial transcriptomics using photoactivatable cell dyes.

IF: 17.694

Cited by: 15

Abstract

A cell's phenotype and function are influenced by dynamic interactions with its microenvironment. To examine cellular spatiotemporal activity, we developed SPACECAT-Spatially PhotoActivatable Color Encoded Cell Address Tags-to annotate, track, and isolate cells while preserving viability. In SPACECAT, samples are stained with photocaged fluorescent molecules, and cells are labeled by uncaging those molecules with user-patterned near-UV light. SPACECAT offers single-cell precision and temporal stability across diverse cell and tissue types. Illustratively, we target crypt-like regions in patient-derived intestinal organoids to enrich for stem-like and actively mitotic cells, matching literature expectations. Moreover, we apply SPACECAT to ex vivo tissue sections from four healthy organs and an autochthonous lung tumor model. Lastly, we provide a computational framework to identify spatially-biased transcriptome patterns and enriched phenotypes. This minimally perturbative and broadly applicable method links cellular spatiotemporal and/or behavioral phenotypes with diverse downstream assays, enabling insights into the connections between tissue microenvironments and (dys)function.

Keywords

Spatial Transcriptomics

MeSH terms

Animals

Biological Assay

Cell Tracking

Coloring Agents

Cytokines

Female

Fluoresceins

Fluorescent Dyes

HEK293 Cells

Health Status

Humans

Lung Neoplasms

Male

Mice

Myeloid Cells

Organoids

Phenotype

Stem Cells

Transcriptome

Tumor Microenvironment

Ultraviolet Rays

Authors

Genshaft, Alex S

Ziegler, Carly G K

Tzouanas, Constantine N

Mead, Benjamin E

Jaeger, Alex M

Navia, Andrew W

King, Ryan P

Mana, Miyeko D

Huang, Siyi

Mitsialis, Vanessa

Snapper, Scott B

Yilmaz, Ömer H

Jacks, Tyler

Van Humbeck, Jeffrey F

Shalek, Alex K

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