PLoS Pathogens (Oct 2023)

Tyrosine phosphorylation of IRF3 by BLK facilitates its sufficient activation and innate antiviral response.

  • Wei-Wei Li,
  • Xu-Xu Fan,
  • Zi-Xiang Zhu,
  • Xue-Jing Cao,
  • Zhao-Yu Zhu,
  • Dan-Shi Pei,
  • Yi-Zhuo Wang,
  • Ji-Yan Zhang,
  • Yan-Yi Wang,
  • Hai-Xue Zheng

DOI
https://doi.org/10.1371/journal.ppat.1011742
Journal volume & issue
Vol. 19, no. 10
p. e1011742

Abstract

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Viral infection triggers the activation of transcription factor IRF3, and its activity is precisely regulated for robust antiviral immune response and effective pathogen clearance. However, how full activation of IRF3 is achieved has not been well defined. Herein, we identified BLK as a key kinase that positively modulates IRF3-dependent signaling cascades and executes a pre-eminent antiviral effect. BLK deficiency attenuates RNA or DNA virus-induced ISRE activation, interferon production and the cellular antiviral response in human and murine cells, whereas overexpression of BLK has the opposite effects. BLK-deficient mice exhibit lower serum cytokine levels and higher lethality after VSV infection. Moreover, BLK deficiency impairs the secretion of downstream antiviral cytokines and promotes Senecavirus A (SVA) proliferation, thereby supporting SVA-induced oncolysis in an in vivo xenograft tumor model. Mechanistically, viral infection triggers BLK autophosphorylation at tyrosine 309. Subsequently, activated BLK directly binds and phosphorylates IRF3 at tyrosine 107, which further promotes TBK1-induced IRF3 S386 and S396 phosphorylation, facilitating sufficient IRF3 activation and downstream antiviral response. Collectively, our findings suggest that targeting BLK enhances viral clearance via specifically regulating IRF3 phosphorylation by a previously undefined mechanism.