AUTHOR=Li Ling , Zhao Manzhi , Kiernan Caoimhe H. , Castro Eiro Melisa D. , van Meurs Marjan , Brouwers-Haspels Inge , Wilmsen Merel E. P. , Grashof Dwin G. B. , van de Werken Harmen J. G. , Hendriks Rudi W. , Mueller Yvonne M. , Katsikis Peter D. 

TITLE=Ibrutinib directly reduces CD8+T cell exhaustion independent of BTK

JOURNAL=Frontiers in Immunology

VOLUME=14

YEAR=2023

URL=https://www.frontiersin.org/journals/immunology/articles/10.3389/fimmu.2023.1201415

DOI=10.3389/fimmu.2023.1201415

ISSN=1664-3224

ABSTRACT=<sec><title>Introduction</title><p>Cytotoxic CD8+ T cell (CTL) exhaustion is a dysfunctional state of T cells triggered by persistent antigen stimulation, with the characteristics of increased inhibitory receptors, impaired cytokine production and a distinct transcriptional profile. Evidence from immune checkpoint blockade therapy supports that reversing T cell exhaustion is a promising strategy in cancer treatment. Ibrutinib, is a potent inhibitor of BTK, which has been approved for the treatment of chronic lymphocytic leukemia. Previous studies have reported improved function of T cells in ibrutinib long-term treated patients but the mechanism remains unclear. We investigated whether ibrutinib directly acts on CD8+ T cells and reinvigorates exhausted CTLs. </p></sec><sec><title>Methods</title><p>We used an established <italic>in vitro</italic> CTL exhaustion system to examine whether ibrutinib can directly ameliorate T cell exhaustion. Changes in inhibitory receptors, transcription factors, cytokine production and killing capacity of ibrutinib-treated exhausted CTLs were detected by flow cytometry. RNA-seq was performed to study transcriptional changes in these cells. Btk deficient mice were used to confirm that the effect of ibrutinib was independent of BTK expression.</p></sec><sec><title>Results</title><p>We found that ibrutinib reduced exhaustion-related features of CTLs in an <italic>in vitro</italic> CTL exhaustion system. These changes included decreased inhibitory receptor expression, enhanced cytokine production, and downregulation of the transcription factor TOX with upregulation of TCF1. RNA-seq further confirmed that ibrutinib directly reduced the exhaustion-related transcriptional profile of these cells. Importantly, using btk deficient mice we showed the effect of ibrutinib was independent of BTK expression, and therefore mediated by one of its other targets. </p></sec><sec><title>Discussion</title><p>Our study demonstrates that ibrutinib directly ameliorates CTL exhaustion, and provides evidence for its synergistic use with cancer immunotherapy.</p></sec>