ESCRT-dependent STING degradation curtails steady-state and cGAMP-induced signaling

Author:

Gentili MatteoORCID,Liu BingxuORCID,Papanastasiou MalvinaORCID,Dele-Oni Deborah,Schwartz Marc AORCID,Carlson Rebecca J.ORCID,Al’Khafaji AzizORCID,Krug KarstenORCID,Brown Adam,Doench John GORCID,Carr Steven AORCID,Hacohen NirORCID

Abstract

AbstractSTING is an intracellular sensor of cyclic di-nucleotides involved in response to pathogen- or self-derived DNA that induces protective immunity, or if dysregulated, autoimmunity. STING trafficking is tightly linked to its activity. We aimed to systematically characterize genes regulating STING trafficking and to define their impact on STING responses. Based on proximity-ligation proteomics and genetic screens, an ESCRT complex containing HGS, VPS37A and UBAP1 was found to be required for STING degradation and signaling shutdown. Analogous to phosphorylated STING creating a platform for IRF3 recruitment, oligomerization-driven STING ubiquitination by UBE2N formed a platform for ESCRT recruitment at the endosome, responsible for STING signaling shutdown. A UBAP1 mutant that underlies human spastic paraplegia and disrupts ESCRT function led to STING-dependent type I IFN responses at the steady-state, defining ESCRT as a homeostatic regulator of STING signaling.

Publisher

Cold Spring Harbor Laboratory

Cited by 2 articles. 订阅此论文施引文献 订阅此论文施引文献,注册后可以免费订阅5篇论文的施引文献,订阅后可以查看论文全部施引文献

1. STING is ESCRTed to degradation by microautophagy;Nature Cell Biology;2023-03

2. STING trafficking as a new dimension of immune signaling;Journal of Experimental Medicine;2023-01-27

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