Endoplasmic reticulum chaperones stabilize ligand-receptive MR1 molecules for efficient presentation of metabolite antigens

Author:

McWilliam Hamish E. G.ORCID,Mak Jeffrey Y. W.ORCID,Awad WaelORCID,Zorkau Matthew,Cruz-Gomez Sebastian,Lim Hui Jing,Yan YutingORCID,Wormald Sam,Dagley Laura F.ORCID,Eckle Sidonia B. G.ORCID,Corbett Alexandra J.ORCID,Liu HaiyinORCID,Li Shihan,Reddiex Scott J. J.ORCID,Mintern Justine D.ORCID,Liu LigongORCID,McCluskey JamesORCID,Rossjohn JamieORCID,Fairlie David P.ORCID,Villadangos Jose A.ORCID

Abstract

The antigen-presenting molecule MR1 (MHC class I-related protein 1) presents metabolite antigens derived from microbial vitamin B2 synthesis to activate mucosal-associated invariant T (MAIT) cells. Key aspects of this evolutionarily conserved pathway remain uncharacterized, including where MR1 acquires ligands and what accessory proteins assist ligand binding. We answer these questions by using a fluorophore-labeled stable MR1 antigen analog, a conformation-specific MR1 mAb, proteomic analysis, and a genome-wide CRISPR/Cas9 library screen. We show that the endoplasmic reticulum (ER) contains a pool of two unliganded MR1 conformers stabilized via interactions with chaperones tapasin and tapasin-related protein. This pool is the primary source of MR1 molecules for the presentation of exogenous metabolite antigens to MAIT cells. Deletion of these chaperones reduces the ER-resident MR1 pool and hampers antigen presentation and MAIT cell activation. The MR1 antigen-presentation pathway thus co-opts ER chaperones to fulfill its unique ability to present exogenous metabolite antigens captured within the ER.

Funder

Australian Research Council

Department of Health | National Health and Medical Research Council

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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