Phosphorylation of IRF8 in a pre-associated complex with Spi-1/PU. 1 and non-phosphorylated Stat1 is critical for LPS induction of the IL1B gene
Molecular immunology, 2007•Elsevier
Rapid induction of transcription is known to be mediated by factors which bind DNA
following post-translational modification. We report here that non-tyrosine phosphorylated
(NTP)-Stat1 is involved in a cooperative interaction with Spi-1/PU. 1 and IRF8 to form a pre-
associated, poised complex for IL1B gene induction. A double point mutation at a putative
STAT binding site, which overlaps this composite Spi-1· IRF8 site located in the LPS and IL-
1 response element (LILRE), inhibited human IL1B LPS-dependent reporter activity to about …
following post-translational modification. We report here that non-tyrosine phosphorylated
(NTP)-Stat1 is involved in a cooperative interaction with Spi-1/PU. 1 and IRF8 to form a pre-
associated, poised complex for IL1B gene induction. A double point mutation at a putative
STAT binding site, which overlaps this composite Spi-1· IRF8 site located in the LPS and IL-
1 response element (LILRE), inhibited human IL1B LPS-dependent reporter activity to about …
Rapid induction of transcription is known to be mediated by factors which bind DNA following post-translational modification. We report here that non-tyrosine phosphorylated (NTP)-Stat1 is involved in a cooperative interaction with Spi-1/PU.1 and IRF8 to form a pre-associated, poised complex for IL1B gene induction. A double point mutation at a putative STAT binding site, which overlaps this composite Spi-1·IRF8 site located in the LPS and IL-1 response element (LILRE), inhibited human IL1B LPS-dependent reporter activity to about 10 percent of the control wild type vector. Chromatin immunoprecipitation revealed stimulation-independent constitutive binding of IRF8, Spi-1 and NTP-Stat1 at the LILRE, while binding of C/EBPβ was activated at an adjacent C/EBPβ site after LPS stimulation. In contrast to Stat1, IRF8 was tyrosine phosphorylated following LPS treatment. Supporting the involvement of NTP-Stat1, LPS-induced IL1B reporter activity in monocytes was enhanced by ectopic expression of NTP-Stat1 Y701F. In contrast, co-expression of a Y211F IRF8 mutein functioned as a dominant-negative inhibitor of LPS-induced IL1B reporter activity. In vitro DNA binding using extracts from LPS-treated monocytes confirmed that the LILRE enhancer constitutively binds a trimolecular complex containing IRF8, Spi-1 and NTP-Stat1. Binding studies using in vitro-expressed proteins revealed that NTP-Stat1 enhanced the binding of Spi-1 and IRF8 to the LILRE. Co-expression of TRAF6, an LPS surrogate, with Spi-1 and IRF8 enhanced IL1B reporter activity in HEK293R cells, which was dramatically reduced when Y211F IRF8 was co-expressed. These results suggest that the rapid transcriptional induction of an important inflammatory gene is dependent upon constitutive cooperative binding of a Spi-1·IRF8·NTP-Stat1 complex to the LILRE, which primes the gene for immediate induction following IRF8 phosphorylation. Phosphorylation of chromatin pre-associated factors like IRF8 may be an important strategy for the rapid transcriptional activation of genes involved in innate immunity.
Elsevier