Ex vivo enrichment of PRAME antigen‐specific T cells for adoptive immunotherapy using CD137 activation marker selection

Koon H Lee; Kavitha Gowrishankar; Janine Street; Helen M McGuire; Fabio Luciani; Brendan Hughes; Mandeep Singh; Leighton E Clancy; David J Gottlieb; Kenneth P Micklethwaite; Emily Blyth

doi:10.1002/cti2.1200

Clinical & Translational Immunology (Jan 2020)

Ex vivo enrichment of PRAME antigen‐specific T cells for adoptive immunotherapy using CD137 activation marker selection

Koon H Lee,
Kavitha Gowrishankar,
Janine Street,
Helen M McGuire,
Fabio Luciani,
Brendan Hughes,
Mandeep Singh,
Leighton E Clancy,
David J Gottlieb,
Kenneth P Micklethwaite,
Emily Blyth

Affiliations

Koon H Lee: Westmead Institute for Medical Research Westmead NSW Australia
Kavitha Gowrishankar: Westmead Institute for Medical Research Westmead NSW Australia
Janine Street: Westmead Institute for Medical Research Westmead NSW Australia
Helen M McGuire: Faculty of Medicine and Health Sydney Medical School Sydney NSW Australia
Fabio Luciani: The Kirby Institute University of New South Wales Darlinghurst NSW Australia
Brendan Hughes: The Kirby Institute University of New South Wales Darlinghurst NSW Australia
Mandeep Singh: The Garvan Institute of Medical Research Darlinghurst NSW Australia
Leighton E Clancy: Westmead Institute for Medical Research Westmead NSW Australia
David J Gottlieb: Westmead Institute for Medical Research Westmead NSW Australia
Kenneth P Micklethwaite: Westmead Institute for Medical Research Westmead NSW Australia
Emily Blyth: Westmead Institute for Medical Research Westmead NSW Australia

DOI: https://doi.org/10.1002/cti2.1200
Journal volume & issue: Vol. 9, no. 10
pp. n/a – n/a

Abstract

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Abstract Objective Adoptive immunotherapy with ex vivo expanded tumor‐specific T cells has potential as anticancer therapy. Preferentially expressed antigen in melanoma (PRAME) is an attractive target overexpressed in several cancers including melanoma and acute myeloid leukaemia (AML), with low expression in normal tissue outside the gonads. We developed a GMP‐compliant manufacturing method for PRAME‐specific T cells from healthy donors for adoptive immunotherapy. Methods Mononuclear cells were pulsed with PRAME 15‐mer overlapping peptide mix. After 16 h, activated cells expressing CD137 were isolated with immunomagnetic beads and cocultured with irradiated CD137neg fraction in medium supplemented with interleukin (IL)‐2, IL‐7 and IL‐15. Cultured T cells were restimulated with antigen‐pulsed autologous cells after 10 days. Cellular phenotype and cytokine response following antigen re‐exposure were assessed with flow cytometry, enzyme‐linked immunospot (ELISPOT) and supernatant cytokine detection. Detailed phenotypic and functional analysis with mass cytometry and T‐cell receptor (TCR) beta clonality studies were performed on selected cultures. Results PRAME‐stimulated cultures (n = 10) had mean expansion of 2500‐fold at day 18. Mean CD3+ percentage was 96% with CD4:CD8 ratio of 4:1. Re‐exposure to PRAME peptide mixture showed enrichment of CD4 cells expressing interferon (IFN)‐γ (mean: 12.2%) and TNF‐α (mean: 19.7%). Central and effector memory cells were 23% and 72%, respectively, with 24% T cells expressing PD1. Mass cytometry showed predominance of Th1 phenotype (CXCR3+/CCR4neg/CCR6neg/Tbet+, mean: 73%) and cytokine production including IL‐2, IL‐4, IL‐8, IL‐13 and GM‐CSF (2%, 6%, 8%, 4% and 11%, respectively). Conclusion PRAME‐specific T cells for adoptive immunotherapy were enriched from healthy donor mononuclear cells. The products were oligoclonal, exhibited Th1 phenotype and produced multiple cytokines.

Published in Clinical & Translational Immunology

ISSN: 2050-0068 (Online)
Publisher: Wiley
Country of publisher: Australia
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Immunologic diseases. Allergy
Website: https://onlinelibrary.wiley.com/journal/20500068

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