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Profiling T cell activation using single-molecule fluorescence in situ hybridization and flow cytometry
Journal article   Peer reviewed

Profiling T cell activation using single-molecule fluorescence in situ hybridization and flow cytometry

Yuri Bushkin, Felix Radford, Richard Pine, Alfred Lardizabal, Bonita T Mangura, Maria Laura Gennaro and Sanjay Tyagi
The Journal of immunology (1950), Vol.194(2), pp.836-841
01/15/2015
PMID: 25505292

Abstract

Adult Aged Antigens, Bacterial - immunology Cytokines - blood Cytokines - immunology Female Flow Cytometry - methods Humans In Situ Hybridization, Fluorescence - methods Lymphocyte Activation Male Middle Aged RNA, Messenger - blood RNA, Messenger - immunology T-Lymphocytes - immunology T-Lymphocytes - pathology Tuberculosis, Pulmonary - blood Tuberculosis, Pulmonary - immunology Tuberculosis, Pulmonary - pathology
Flow cytometric characterization of Ag-specific T cells typically relies on detection of protein analytes. Shifting the analysis to detection of RNA would provide several significant advantages, which we illustrate by developing a new host immunity-based platform for detection of infections. Cytokine mRNAs synthesized in response to ex vivo stimulation with pathogen-specific Ags are detected in T cells with single-molecule fluorescence in situ hybridization followed by flow cytometry. Background from pre-existing in vivo analytes is lower for RNAs than for proteins, allowing greater sensitivity for detection of low-frequency cells. Moreover, mRNA analysis reveals kinetic differences in cytokine expression that are not apparent at the protein level but provide novel insights into gene expression programs expected to define different T cell subsets. The utility of probing immunological memory of infections is demonstrated by detecting T cells that recognize mycobacterial and viral Ags in donors exposed to the respective pathogens.
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https://doi.org/10.4049/jimmunol.1401515View
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