Selective SIK2/SIK3 inhibition reprograms pro- and antiinflammatory pathways in myeloid cells, improving autoimmune disease outcomes
Steve De Vos, Nicolas Desroy, Susan J. Bellaire, Anna Pereira Fernandes, Stéphanie Lavazais, Didier Merciris, Carole Delachaume, Catherine Robin-Jagerschmidt, Adrien Cosson, Angela Lazaryan, Nancy Van Osselaer, David Amantini, Christophe Peixoto, Maikel L. Colli, Thomas Van Eeckhoutte, Tiina Hakonen, Magali Constant, Alberto Garcia-Hernandez, Rahul Barron, Geert D’Haens, Wulf O. Böcher
Steve De Vos, Nicolas Desroy, Susan J. Bellaire, Anna Pereira Fernandes, Stéphanie Lavazais, Didier Merciris, Carole Delachaume, Catherine Robin-Jagerschmidt, Adrien Cosson, Angela Lazaryan, Nancy Van Osselaer, David Amantini, Christophe Peixoto, Maikel L. Colli, Thomas Van Eeckhoutte, Tiina Hakonen, Magali Constant, Alberto Garcia-Hernandez, Rahul Barron, Geert D’Haens, Wulf O. Böcher
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Research Article Dermatology Gastroenterology

Selective SIK2/SIK3 inhibition reprograms pro- and antiinflammatory pathways in myeloid cells, improving autoimmune disease outcomes

Abstract

Adaptive immune responses are widely considered the primary drivers of chronic inflammation in autoimmune disease, yet increasing evidence suggests that dysregulated myeloid cells play a central role in sustaining tissue damage. Salt-inducible kinases (SIKs) regulate immune cell activation, and their pharmacological inhibition can promote a shift from proinflammatory toward an immunoregulatory phenotype. We investigated whether selective inhibition of SIK2 and SIK3 with GLPG3970 could reprogram monocytes, macrophages, and dendritic cells, and we assessed pharmacological effects on activated T and B cells. Preclinical studies in mouse models of colitis, psoriasis, and arthritis demonstrated that SIK2/SIK3 inhibition reduced inflammatory activity and promoted immunoregulatory and tolerogenic-associated pathways. Clinical signal-detection studies in ulcerative colitis, psoriasis, and rheumatoid arthritis revealed signs of clinical and biological activity in ulcerative colitis and psoriasis. These findings suggest that myeloid cell dysfunction and impaired myeloid phenotype switching contribute to chronic inflammation in autoimmune diseases and that therapeutic targeting of SIK2/SIK3 holds the potential to restore immune balance by converting proinflammatory into regulatory pathways. Collectively, this work supports SIK2/SIK3 inhibition as a potential treatment strategy for myeloid cell–driven chronic inflammatory conditions.

Authors

Steve De Vos, Nicolas Desroy, Susan J. Bellaire, Anna Pereira Fernandes, Stéphanie Lavazais, Didier Merciris, Carole Delachaume, Catherine Robin-Jagerschmidt, Adrien Cosson, Angela Lazaryan, Nancy Van Osselaer, David Amantini, Christophe Peixoto, Maikel L. Colli, Thomas Van Eeckhoutte, Tiina Hakonen, Magali Constant, Alberto Garcia-Hernandez, Rahul Barron, Geert D’Haens, Wulf O. Böcher

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Figure 2

GLPG3970 induces tolerogenic DCs.

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GLPG3970 induces tolerogenic DCs. (A) Inhibition of TNF-α and IL-12p40 a...
(A) Inhibition of TNF-α and IL-12p40 and induction of IL-10, THBS1, and AREG by GLPG3970 in LPS-stimulated human monocyte-derived DCs. After differentiation, DCs were treated with GLPG3970 at 20, 6.7, 2.2, 0.74, 0.25, or 0.08 μM. Cytokines were measured at 24 hours after LPS stimulation, except for IL-10 (4 hours). Data were collected from 2 independent donors, each with 2 biological replicates. (B) Expression of DC surface markers (ILT4, CD163, CD209, HLA-DR) on CD14+CD11c+ cells after 5 days of differentiation in the presence of 2.2 μM GLPG3970. Data are presented as mean values from 2 donors. (C) Percentage inhibition of TNF-α, IL-12p40, IL-6, and IL-23 and fold induction of IL-10 in LPS-stimulated DCs differentiated in the presence of GLPG3970 (2.2, 0.7, 0.2, 0.08, 0.03, 0.001 μM). Cytokines were measured 4 hours after LPS stimulation. Sample sizes: n = 8 donors for TNF-α, IL-12p40, IL-6, and IL-10; n = 5 for IL-23. Statistical comparisons: (B) GLPG3970 vs. vehicle by paired t test with FDR correction; (A and C) 1-way ANOVA with Dunnett’s multiple comparisons vs. LPS controls. ####P < 0.0001; nsP > 0.05; *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. AREG, amphiregulin; HLA-DR, human leukocyte antigen–DR isotype; ILT4, immunoglobulin-like transcript 4; THBS1, thrombospondin 1.