A stress sensor IRE1α is required for bacterial exotoxin-induced inflammasome activation in tissue-resident macrophages

Author:

Sasaki IzumiORCID,Fukuda-Ohta Yuri,Nakai Chihiro,Wakaki-Nishiyama Naoko,Okamoto Chizuyo,Orimo Takashi,Okuzaki Daisuke,Morita Shuhei,Kaji Shiori,Furuta Yuki,Hemmi Hiroaki,Kato Takashi,Yamamoto Asumi,Tanaka Takashi,Hoshino Katsuaki,Fukuda Shinji,Miyake Kensuke,Kuroda Etsushi,Ishii Ken J.ORCID,Iwawaki Takao,Furukawa Koichi,Kaisho Tsuneyasu

Abstract

AbstractCholera toxin (CT), a bacterial exotoxin composed of one A subunit (CTA) and five B subunits (CTB), functions as an immune adjuvant. CTB can induce production of interleukin-1β (IL-1β), a proinflammatory cytokine, in synergy with a lipopolysaccharide (LPS), from resident peritoneal macrophages (RPMs) through the pyrin and NLRP3 inflammasomes. However, how CTB or CT activates these inflammasomes in the macrophages has been unclear. Here, we clarified the roles of IRE1α, an endoplasmic reticulum (ER) stress sensor, in CT-induced IL-1β production from RPMs. In RPMs, CTB is incorporated into ER and induced ER stress responses, depending on GM1, a cell membrane ganglioside. IRE1α-deficient RPMs showed a significant impairment of CT- or CTB-induced IL-1β production, indicating that IRE1α was required for CT- or CTB-induced IL-1β production from RPMs. This study first demonstrates the critical roles of IRE1α in activation of both NLRP3 and pyrin inflammasomes in tissue-resident macrophages.One sentence summaryIRE1α is required for NLRP3 and pyrin-mediated IL-1β production

Publisher

Cold Spring Harbor Laboratory

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