Rapid selection and identification of functional CD8 T cell epitopes from large peptide-coding libraries.

Nat Commun

Michael Smith Genome Sciences Centre, British Columbia Cancer Agency, 675W 10th Ave, Vancouver, BC, V5Z 1L3, Canada.

Published: October 2019

Cytotoxic CD8 T cells recognize and eliminate infected or malignant cells that present peptide epitopes derived from intracellularly processed antigens on their surface. However, comprehensive profiling of specific major histocompatibility complex (MHC)-bound peptide epitopes that are naturally processed and capable of eliciting a functional T cell response has been challenging. Here, we report a method for deep and unbiased T cell epitope profiling, using in vitro co-culture of CD8 T cells together with target cells transduced with high-complexity, epitope-encoding minigene libraries. Target cells that are subject to cytotoxic attack from T cells in co-culture are isolated prior to apoptosis by fluorescence-activated cell sorting, and characterized by sequencing the encoded minigenes. We then validate this highly parallelized method using known murine T cell receptor/peptide-MHC pairs and diverse minigene-encoded epitope libraries. Our data thus suggest that this epitope profiling method allows unambiguous and sensitive identification of naturally processed and MHC-presented peptide epitopes.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6779888PMC
http://dx.doi.org/10.1038/s41467-019-12444-7DOI Listing

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