Regnase-1 degradation is crucial for IL-33- and IL-25-mediated ILC2 activation.

Kazufumi Matsushita,Shizuo Akira,Shoko Akasaki,Hiroki Tanaka,Takumi Adachi,Koubun Yasuda,Tomohiro Yoshimoto,Atsuhide Koida,Ayumi Fukuoka,Etsushi Kuroda

doi:10.1172/jci.insight.131480

Abstract

Group 2 innate lymphoid cells (ILC2s) are a critical innate source of type 2 cytokines in allergic inflammation. Although ILC2s are recognized as a critical cell population in the allergic inflammation, the regulatory mechanism(s) of ILC2s are less well understood. Here, we show that Regnase-1, an immune regulatory RNAse that degrades inflammatory mRNAs, negatively regulates ILC2 function and that IκB kinase (IKK) complex-mediated Regnase-1 degradation is essential for IL-33- and IL-25-induced ILC2 activation. ILC2s from Regnase-1AA/AA mice expressing a Regnase-1 S435A/S439A mutant resistant to IKK complex-mediated degradation accumulated Regnase-1 protein in response to IL-33 and IL-25. IL-33- and IL-25-stimulated Regnase-1AA/AA ILC2s showed reduced cell proliferation and type 2 cytokine (IL-5, IL-9, and IL-13) production and increased cell death. In addition, Il2ra and Il1rl1, but not Il5, Il9, or Il13, mRNAs were destabilized in IL-33-stimulated Regnase-1AA/AA ILC2s. In vivo, Regnase-1AA/AA mice showed attenuated acute type 2 pulmonary inflammation induced by the instillation of IL-33, IL-25, or papain. Furthermore, the expulsion of Nippostrongylus brasiliensis was significantly delayed in Regnase-1AA/AA mice. These results demonstrate that IKK complex-mediated Regnase-1 degradation is essential for ILC2-mediated type 2 responses both in vitro and in vivo. Therefore, controlling Regnase-1 degradation is a potential therapeutic target for ILC2-contributed allergic disorders.

Highlights

Group 2 innate lymphoid cells (ILC2s) produce a large quantity of type 2 cytokines, including IL-5, IL-9, and IL-13, and are considered an innate counterpart of Th2 cells [1,2,3,4]
We show that Regnase-1 undergoes S435/S439 motif–dependent degradation downstream of IL-33 and IL-25 and that Regnase-1 degradation is crucial for IL-33– and IL-25–induced ILC2 activation both in vitro and in vivo
Regnase-1 is phosphorylated at S494/S513 by TANK-binding kinase 1 (TBK1) and inducible IKK (IKKi) downstream of IL-17 [23], slowly migrating Regnase-1 was not detected in IL-2/25–stimulated ILC2s

Summary

Introduction

Group 2 innate lymphoid cells (ILC2s) produce a large quantity of type 2 cytokines, including IL-5, IL-9, and IL-13, and are considered an innate counterpart of Th2 cells [1,2,3,4]. ILC2s do not express a specific antigen receptor but quickly respond to epithelial cell–derived cytokines, such as IL-33 and IL-25 ( known as IL-17E) [4]. This epithelial cytokine-mediated ILC2 activation is sufficient to induce allergic pulmonary inflammation evoked by the instillation of papain [5, 6], house dust mite [7, 8], or Alternaria alternata [9, 10] in mice. A deeper understanding of the regulatory mechanisms of ILC2 activation is essential to develop therapeutic measures for type 2 immunity-associated disorders

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Conclusion