STING signalling is terminated through ESCRT-dependent microautophagy of vesicles originating from recycling endosomes

细胞生物学 内体 ESCRT公司 高尔基体 干扰素基因刺激剂 生物 溶酶体 TSG101型 内质网 液泡 先天免疫系统 微泡 生物化学 细胞质 基因 细胞内 小RNA 受体 航空航天工程 工程类
作者
Yoshihiko Kuchitsu,Kojiro Mukai,Rei Uematsu,Yuki Takaada,Ayumi Shinojima,Ruri Shindo,Tsumugi Shoji,Shiori Hamano,Emari Ogawa,Ryôsuke Satô,Kensuke Miyake,Akira Kato,Yasushi Kawaguchi,Masahiko Nishitani‐Isa,Kazushi Izawa,Ryuta Nishikomori,Takahiro Yasumi,Takehiro Suzuki,Naoshi Dohmae,Takefumi Uemura,Glen N. Barber,Hiroyuki Arai,Satoshi Waguri,Tomohiko Taguchi
出处
期刊:Nature Cell Biology [Springer Nature]
卷期号:25 (3): 453-466 被引量:22
标识
DOI:10.1038/s41556-023-01098-9
摘要

Stimulator of interferon genes (STING) is essential for the type I interferon response against a variety of DNA pathogens. Upon emergence of cytosolic DNA, STING translocates from the endoplasmic reticulum to the Golgi where STING activates the downstream kinase TBK1, then to lysosome through recycling endosomes (REs) for its degradation. Although the molecular machinery of STING activation is extensively studied and defined, the one underlying STING degradation and inactivation has not yet been fully elucidated. Here we show that STING is degraded by the endosomal sorting complexes required for transport (ESCRT)-driven microautophagy. Airyscan super-resolution microscopy and correlative light/electron microscopy suggest that STING-positive vesicles of an RE origin are directly encapsulated into Lamp1-positive compartments. Screening of mammalian Vps genes, the yeast homologues of which regulate Golgi-to-vacuole transport, shows that ESCRT proteins are essential for the STING encapsulation into Lamp1-positive compartments. Knockdown of Tsg101 and Vps4, components of ESCRT, results in the accumulation of STING vesicles in the cytosol, leading to the sustained type I interferon response. Knockdown of Tsg101 in human primary T cells leads to an increase the expression of interferon-stimulated genes. STING undergoes K63-linked ubiquitination at lysine 288 during its transit through the Golgi/REs, and this ubiquitination is required for STING degradation. Our results reveal a molecular mechanism that prevents hyperactivation of innate immune signalling, which operates at REs.
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