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A versatile T cell-based assay to assess therapeutic antigenspecific PD-1-targeted approaches
Tijdschriftbijdrage - Tijdschriftartikel
Blockade of programmed cell death protein 1 (PD-1) immune checkpoint
receptor signaling is an established standard treatment for many types of cancer
and indications are expanding. Successful clinical trials using monoclonal antibodies
targeting PD-1 signaling have boosted preclinical research, encouraging development
of novel therapeutics. Standardized assays to evaluate their bioactivity, however,
remain restricted. The robust bioassays available all lack antigen-specificity. Here,
we developed an antigen-specific, short-term and high-throughput T cell assay with
versatile readout possibilities. A genetically modified T cell receptor (TCR)-deficient T
cell line was stably transduced with PD-1. Transfection with messenger RNA encoding
a TCR of interest and subsequent overnight stimulation with antigen-presenting
cells, results in eGFP-positive and granzyme B-producing T cells for single cell or
bulk analysis. Control antigen-presenting cells induced reproducible high antigenspecific
eGFP and granzyme B expression. Upon PD-1 interaction, ligand-positive
antigen-presenting immune or tumor cells elicited significantly lower eGFP and
granzyme B expression, which could be restored by anti-PD-(L)1 blocking antibodies.
This convenient cell-based assay shows a valuable tool for translational and clinical
research on antigen-specific checkpoint-targeted therapy approaches.
receptor signaling is an established standard treatment for many types of cancer
and indications are expanding. Successful clinical trials using monoclonal antibodies
targeting PD-1 signaling have boosted preclinical research, encouraging development
of novel therapeutics. Standardized assays to evaluate their bioactivity, however,
remain restricted. The robust bioassays available all lack antigen-specificity. Here,
we developed an antigen-specific, short-term and high-throughput T cell assay with
versatile readout possibilities. A genetically modified T cell receptor (TCR)-deficient T
cell line was stably transduced with PD-1. Transfection with messenger RNA encoding
a TCR of interest and subsequent overnight stimulation with antigen-presenting
cells, results in eGFP-positive and granzyme B-producing T cells for single cell or
bulk analysis. Control antigen-presenting cells induced reproducible high antigenspecific
eGFP and granzyme B expression. Upon PD-1 interaction, ligand-positive
antigen-presenting immune or tumor cells elicited significantly lower eGFP and
granzyme B expression, which could be restored by anti-PD-(L)1 blocking antibodies.
This convenient cell-based assay shows a valuable tool for translational and clinical
research on antigen-specific checkpoint-targeted therapy approaches.
Tijdschrift: Oncotarget
ISSN: 1949-2553
Issue: 45
Volume: 9
Pagina's: 27797-27808
Jaar van publicatie:2018
Auteurs:International
Toegankelijkheid:Open