Characterization and clinical enrichment of HLA-C*07:02-restricted Cytomegalovirus-specific CD8+ T cells | Zendy

Fabian Schlott | Zendy; Dominik Steubl | Zendy; Stefanie Ameres | Zendy; Andreas Moosmann | Zendy; Stefan Dreher | Zendy; Uwe Heemann | Zendy; Volker Hösel | Zendy; Dirk H. Busch | Zendy; Michael Neuenhahn | Zendy

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Characterization and clinical enrichment of HLA-C*07:02-restricted Cytomegalovirus-specific CD8+ T cells

Author(s) -

Fabian Schlott,

Dominik Steubl,

Stefanie Ameres,

Andreas Moosmann,

Stefan Dreher,

Uwe Heemann,

Volker Hösel,

Dirk H. Busch,

Michael Neuenhahn

Publication year - 2018

Publication title -

plos one

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.99

H-Index - 332

ISSN - 1932-6203

DOI - 10.1371/journal.pone.0193554

Subject(s) - epitope , human leukocyte antigen , cd8 , t cell , cytotoxic t cell , immunology , immune system , virology , biology , transplantation , major histocompatibility complex , hla a , antigen , medicine , genetics , in vitro

Human Cytomegalovirus (CMV) reactivation remains a major source of morbidity in patients after solid organ and hematopoietic stem cell transplantation (HSCT). Adoptive T cell therapy (ACT) with CMV-specific T cells is a promising therapeutic approach for HSCT recipients, but might be counteracted by CMV’s immune evasion strategies. HLA-C*07:02 is less susceptible to viral immune evasion suggesting HLA-C*07:02-restricted viral epitopes as promising targets for ACT. For a better understanding of HLA-C*07:02-restricted CMV-specific T cells we used recently generated reversible HLA-C*07:02/IE-1 multimers (Streptamers) recognizing a CMV-derived Immediate-Early-1 (IE-1) epitope and analyzed phenotypic and functional T cell characteristics. Initially, we detected very high frequencies of HLA-C*07:02/IE-1 multimer + T cells (median = 11.35%), as well as robust functional responses after stimulation with IE-1 peptide (IFNγ + ; median = 5.02%) in healthy individuals. However, MHC-multimer + and IFNγ-secreting T cell frequencies showed a relatively weak correlation (r 2 = 0.77), which could be attributed to an unexpected contribution of CMV-epitope-independent KIR2DL2/3-binding of HLA-C*07:02/IE-1 multimers. Therefore, we developed a MHC-multimer double-staining approach against a cancer epitope-specific HLA-C*07:02 multimer to identify truly HLA-C*07:02/IE-1 epitope-specific T cells. The frequencies of these truly HLA-C*07:02/IE-1 multimer + T cells were still high (median = 6.86%) and correlated now strongly (r 2 = 0.96) with IFNγ-secretion. Interestingly, HLA-C*07:02/IE-1-restricted T cells contain substantial numbers with a central memory T cell phenotype, indicating high expansion potential e.g. for ACT. In line with that, we developed a clinical enrichment protocol avoiding epitope-independent KIR-binding to make HLA-C*07:02/IE-1-restricted T cells available for ACT. Initial depletion of KIR-expressing CD8 + T cells followed by HLA-C*07:02/IE-1 Streptamer positive selection using paramagnetic labeling techniques allowed to enrich successfully HLA-C*07:02/IE-1-restricted T cells. Such specifically enriched populations of functional HLA-C*07:02/IE-1-restricted T cells with significant central memory T cell content could become a potent source for ACT.

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