4.7 Article

Dissecting T cell lineage relationships by cellular barcoding

Journal

JOURNAL OF EXPERIMENTAL MEDICINE
Volume 205, Issue 10, Pages 2309-2318

Publisher

ROCKEFELLER UNIV PRESS
DOI: 10.1084/jem.20072462

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Funding

  1. Netherlands Organization for Scientific Research (NWO-Veni) [916.56.155]

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T cells, as well as other cell types, are composed of phenotypically and functionally distinct subsets. However, for many of these populations it is unclear whether they develop from common or separate progenitors. To address such issues, we developed a novel approach, termed cellular barcoding, that allows the dissection of lineage relationships. We demonstrate that the labeling of cells with unique identifiers coupled to a microarray-based detection system can be used to analyze family relationships between the progeny of such cells. To exemplify the potential of this technique, we studied migration patterns of families of antigen-specifi c CD8(+) T cells in vivo. We demonstrate that progeny of individual T cells rapidly seed independent lymph nodes and that antigen-specifi c CD8(+) T cells present at different effector sites are largely derived from a common pool of precursors. These data show how locally primed T cells disperse and provide a technology for kinship analysis with wider utility.

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