The mTORC1-4E-BP-eIF4E axis controls de novo Bcl6 protein synthesis in T cells and systemic autoimmunity

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作者
Woelsung Yi
Sanjay Gupta
Edd Ricker
Michela Manni
Rolf Jessberger
Yurii Chinenov
Henrik Molina
Alessandra B. Pernis
机构
[1] Hospital for Special Surgery,Autoimmunity and Inflammation Program
[2] Weill Cornell Graduate School of Medical Sciences,Graduate Program in Immunology and Microbial Pathogenesis
[3] Technische Universität Dresden,Institute of Physiological Chemistry
[4] Hospital for Special Surgery,Arthritis and Tissue Degeneration Program
[5] Hospital for Special Surgery,David Z. Rosensweig Genomics Research Center
[6] The Rockefeller University,Proteomics Resource Center
[7] Cornell University,Department of Medicine, Weill Cornell Medical College
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Post-transcriptional modifications can control protein abundance, but the extent to which these alterations contribute to the expression of T helper (TH) lineage-defining factors is unknown. Tight regulation of Bcl6 expression, an essential transcription factor for T follicular helper (TFH) cells, is critical as aberrant TFH cell expansion is associated with autoimmune diseases, such as systemic lupus erythematosus (SLE). Here we show that lack of the SLE risk variant Def6 results in deregulation of Bcl6 protein synthesis in T cells as a result of enhanced activation of the mTORC1–4E-BP–eIF4E axis, secondary to aberrant assembly of a raptor–p62–TRAF6 complex. Proteomic analysis reveals that this pathway selectively controls the abundance of a subset of proteins. Rapamycin or raptor deletion ameliorates the aberrant TFH cell expansion in mice lacking Def6. Thus deregulation of mTORC1-dependent pathways controlling protein synthesis can result in T-cell dysfunction, indicating a mechanism by which mTORC1 can promote autoimmunity.
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