Malt1-Induced Cleavage of Regnase-1 in CD4+ Helper T Cells Regulates Immune Activation

نویسندگان

  • Takuya Uehata
  • Hidenori Iwasaki
  • Alexis Vandenbon
  • Kazufumi Matsushita
  • Eduardo Hernandez-Cuellar
  • Kanako Kuniyoshi
  • Takashi Satoh
  • Takashi Mino
  • Yutaka Suzuki
  • Daron M. Standley
  • Tohru Tsujimura
  • Hiromi Rakugi
  • Yoshitaka Isaka
  • Osamu Takeuchi
  • Shizuo Akira
چکیده

Regnase-1 (also known as Zc3h12a and MCPIP1) is an RNase that destabilizes a set of mRNAs, including Il6 and Il12b, through cleavage of their 3' UTRs. Although Regnase-1 inactivation leads to development of an autoimmune disease characterized by T cell activation and hyperimmunoglobulinemia in mice, the mechanism of Regnase-1-mediated immune regulation has remained unclear. We show that Regnase-1 is essential for preventing aberrant effector CD4(+) T cell generation cell autonomously. Moreover, in T cells, Regnase-1 regulates the mRNAs of a set of genes, including c-Rel, Ox40, and Il2, through cleavage of their 3' UTRs. Interestingly, T cell receptor (TCR) stimulation leads to cleavage of Regnase-1 at R111 by Malt1/paracaspase, freeing T cells from Regnase-1-mediated suppression. Furthermore, Malt1 protease activity is critical for controlling the mRNA stability of T cell effector genes. Collectively, these results indicate that dynamic control of Regnase-1 expression in T cells is critical for controlling T cell activation.

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عنوان ژورنال:
  • Cell

دوره 153  شماره 

صفحات  -

تاریخ انتشار 2013