IL-33 activates group 2 innate lymphoid cell expansion and modulates endometriosis
Jessica E. Miller, … , Madhuri Koti, Chandrakant Tayade
Jessica E. Miller, … , Madhuri Koti, Chandrakant Tayade
Published October 26, 2021
Citation Information: JCI Insight. 2021;6(23):e149699. https://doi.org/10.1172/jci.insight.149699.
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Research Article Immunology Reproductive biology

IL-33 activates group 2 innate lymphoid cell expansion and modulates endometriosis

Abstract

Chronic inflammation and localized alterations in immune cell function are suspected to contribute to the progression of endometriosis and its associated symptoms. In particular, the alarmin IL-33 is elevated in the plasma, peritoneal fluid, and endometriotic lesions from patients with endometriosis; however, the exact role of IL-33 in the pathophysiology of endometriosis is not well understood. In this study, we demonstrate, in both humans and a murine model, that IL-33 contributes to the expansion of group 2 innate lymphoid cells (ILC2s), and this IL-33–induced ILC2 expansion modulates the endometriosis lesion microenvironment. Importantly, we show that IL-33 drives hallmarks of severe endometriosis, including elevated inflammation, lesion proliferation, and fibrosis, and that this IL-33–induced aggravation is mediated by ILC2s. Finally, we demonstrate the functionality of IL-33 neutralization as a promising and potentially novel therapeutic avenue for treating the debilitating symptoms of endometriosis.

Authors

Jessica E. Miller, Harshavardhan Lingegowda, Lindsey K. Symons, Olga Bougie, Steven L. Young, Bruce A. Lessey, Madhuri Koti, Chandrakant Tayade

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Figure 8

IL-33 Neutralization represents a promising therapeutic avenue in EMS.

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IL-33 Neutralization represents a promising therapeutic avenue in EMS. W...
WT mice were induced with endometriosis and underwent alternate day i.p. injections of IL-33 along with either a neutralizing IL-33 antibody (αIL-33) (n = 5) or IL-33 and IgG control antibody (αIgG) (n = 5). (A) Cytokine and chemokine analysis in PF samples from αIL-33– or αIgG-treated EMS mice. (B) Peritoneal lavage cells harvested from αIL-33– or αIgG-treated EMS mice counted using a Countess II FL Automated Cell Counter. (C) Frequency of ST2+ cells in the αIL-33– or αIgG-treated WT mice analyzed via flow cytometry. (D) Frequency of eosinophils (singlet, live, CD45+CD11b+F4/80+, Siglec-F+). (E) Frequency of LPM (singlet, live, CD45+CD11b+Siglec-FF4/80hi, MHC-IIlo). (F) Frequency of SPM (singlet, live, CD45+CD11b+Siglec-FF4/80lo, MHC-IIhi). (G) Frequency of ILC2 (singlet, live, CD45+lineageCD25+Thy2+, ST2+). (H) Frequency of Th cells. (I–K) Representative immunohistochemical staining and quantitative analysis of lesion Ki67 staining. (L–N) Representative immunohistochemical staining and quantitative analysis of lesion CD31 staining. (OQ) Representative immunohistochemical staining and analysis of lesion Pgp9.5 staining. (R and S) Representative histochemical staining of lesion Masson’s trichrome staining. Original magnification, ×200. Scale bar: 50 μm. Mean ± SD. Nonparametric Student’s t test with Mann-Whitney.