IL-1 receptor–associated kinase-3 acts as an immune checkpoint in myeloid cells to limit cancer immunotherapy
Gürcan Tunalı, … , Irineos Papakyriacou, Yumeng Mao
Gürcan Tunalı, … , Irineos Papakyriacou, Yumeng Mao
Published February 9, 2023
Citation Information: J Clin Invest. 2023;133(7):e161084. https://doi.org/10.1172/JCI161084.
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Research Article Immunology Oncology

IL-1 receptor–associated kinase-3 acts as an immune checkpoint in myeloid cells to limit cancer immunotherapy

Abstract

Inflammatory mediators released by cancer cells promote the induction of immune suppression and tolerance in myeloid cells. IL-1 receptor–associated kinase-3 (IRAK3) is a pseudokinase that inhibits IL-1/TLR signaling, but its role in patients treated with immune checkpoint blockade (ICB) therapy remains unclear. Using RNA-Seq data from the IMvigor210 trial, we found that tumors with high IRAK3 expressions showed enriched antiinflammatory pathways and worse clinical response to ICB therapy. Upon IRAK3 protein deletion with CRISPR/Cas9, primary human monocytes displayed altered global protein expression and phosphorylation in quantitative proteomics and released more proinflammatory cytokines in response to stimulation. Bone marrow–derived macrophages from an IRAK3 CRISPR KO mouse model demonstrated a proinflammatory phenotype and enhanced sensitivity to TLR agonists compared with WT cells. IRAK3 deficiency delayed the growth of carcinogen-induced and oncogene-driven murine cancer cells and induced enhanced activation in myeloid cells and T cells. Upon ICB treatment, IRAK3-KO mice showed enrichment of TCF1+PD-1+ stem-like memory CD8+ T cells and resulted in superior growth inhibition of immunologically cold tumors in vivo. Altogether, our study demonstrated what we believe to be a novel cancer-driven immune tolerance program controlled by IRAK3 in humans and mice and proposed its suitability as an immunotherapy target.

Authors

Gürcan Tunalı, Marta Rúbies Bedós, Divya Nagarajan, Patrik Fridh, Irineos Papakyriacou, Yumeng Mao

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Figure 3

IRAK3 deletion amplifies signaling through TLR in primary human monocytes.

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IRAK3 deletion amplifies signaling through TLR in primary human monocyte...
(A) Experimental flow for the phospho-proteomics analysis in control or IRAK3-KO primary monocytes isolated from 3 donors. The most significantly changed phosphosites after IRAK3 deletion in monocytes were shown. Detection of phosphorylated proteins using a phospho-kinase array in control or IRAK3 KO (B) THP1 cells or (C) primary human monocytes, in response to 1 μg/mL LPS treatment for 45 minutes. Representative membranes from 2 repeats was shown. (D) Individual detection of pCREB(S133) or pHSP27(S78/82) by ELISA in control or IRAK3-KO THP1 cells in response to increasing concentrations of LPS or Pam3CSK4 for 45 minutes. Data were summarized from 2–5 biological repeats and shown as mean ± SD. Statistical tests were performed using unpaired t tests. *P < 0.05, **P < 0.01, ***P < 0.001.