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ESCRT-dependent STING degradation inhibits steady-state and cGAMP-induced signalling

Author

Listed:
  • Matteo Gentili

    (Broad Institute of MIT and Harvard)

  • Bingxu Liu

    (Broad Institute of MIT and Harvard
    Massachusetts Institute of Technology
    The Koch Institute for Integrative Cancer Research at MIT)

  • Malvina Papanastasiou

    (Broad Institute of MIT and Harvard)

  • Deborah Dele-Oni

    (Broad Institute of MIT and Harvard)

  • Marc A. Schwartz

    (Broad Institute of MIT and Harvard
    Harvard Medical School
    Boston Children’s Hospital
    Dana Farber Cancer Institute)

  • Rebecca J. Carlson

    (Broad Institute of MIT and Harvard
    Massachusetts Institute of Technology, Department of Health Sciences and Technology)

  • Aziz M. Al’Khafaji

    (Broad Institute of MIT and Harvard)

  • Karsten Krug

    (Broad Institute of MIT and Harvard)

  • Adam Brown

    (Broad Institute of MIT and Harvard)

  • John G. Doench

    (Broad Institute of MIT and Harvard)

  • Steven A. Carr

    (Broad Institute of MIT and Harvard)

  • Nir Hacohen

    (Broad Institute of MIT and Harvard
    Massachusetts General Hospital, Harvard Medical School
    Center for Cancer Research, Massachusetts General Hospital)

Abstract

Stimulator of interferon genes (STING) is an intracellular sensor of cyclic di-nucleotides involved in the innate immune response against pathogen- or self-derived DNA. STING trafficking is tightly linked to its function, and its dysregulation can lead to disease. Here, we systematically characterize genes regulating STING trafficking and examine their impact on STING-mediated responses. Using proximity-ligation proteomics and genetic screens, we demonstrate that an endosomal sorting complex required for transport (ESCRT) complex containing HGS, VPS37A and UBAP1 promotes STING degradation, thereby terminating STING-mediated signaling. Mechanistically, STING oligomerization increases its ubiquitination by UBE2N, forming a platform for ESCRT recruitment at the endosome that terminates STING signaling via sorting in the lysosome. Finally, we show that expression of a UBAP1 mutant identified in patients with hereditary spastic paraplegia and associated with disrupted ESCRT function, increases steady-state STING-dependent type I IFN responses in healthy primary monocyte-derived dendritic cells and fibroblasts. Based on these findings, we propose that STING is subject to a tonic degradative flux and that the ESCRT complex acts as a homeostatic regulator of STING signaling.

Suggested Citation

  • Matteo Gentili & Bingxu Liu & Malvina Papanastasiou & Deborah Dele-Oni & Marc A. Schwartz & Rebecca J. Carlson & Aziz M. Al’Khafaji & Karsten Krug & Adam Brown & John G. Doench & Steven A. Carr & Nir , 2023. "ESCRT-dependent STING degradation inhibits steady-state and cGAMP-induced signalling," Nature Communications, Nature, vol. 14(1), pages 1-22, December.
  • Handle: RePEc:nat:natcom:v:14:y:2023:i:1:d:10.1038_s41467-023-36132-9
    DOI: 10.1038/s41467-023-36132-9
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    References listed on IDEAS

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