On the other hand, expression of the M2 marker genes encoding Arg1, Ym1, Fizz1, MR and IL-13 was severely impaired in Jmjd3−/− BM macrophages cultivated in the presence of M-CSF to induce M2 polarization, indicating that Jmjd3 is critical for M2 marker gene expression in BM macrophages. Although M-CSF-induced BM macrophages or chitin-induced peritoneal macrophages showed severe defects in M2 macrophage BGB324 molecular weight marker expression in the absence of Jmjd3, Jmjd3−/− BM macrophages were capable of upregulating expression of genes representative of M2 macrophages in response to IL-4 stimulation. These findings indicate that Jmjd3-mediated H3K27 demethylation is dispensable for the generation
of M2 polarization in response to IL-4, and suggest that M2 macrophages should be further subcategorized depending on the requirement of Jmjd3. Jmjd3 contains an N-terminal tetratricopeptide repeat domain and the JmjC domain in the C-terminus 32–34. The expression of the C-terminal part of Jmjd3 containing the JmjC domain, but not its demethylase-defective mutant, was sufficient to rescue M2 marker expression in Jmjd3−/− BM
macrophages. Therefore, Jmjd3 functions as a demethylase to induce M2 macrophage polarization, although recent studies show PD0325901 a demethylase-independent role in controlling chromatin remodeling together with T-box family transcription factors 40. Chromatin immunoprecipitation-sequencing (ChIP-Seq) analysis revealed that, in general, trimethyl H3K27 was enriched in the promoter regions close to the transcription start sites in BM macrophages. H3K27 of M2 marker genes, such as Arg1, Ym1 and Mrc1, were not trimethylated in the presence RVX-208 or absence of Jmjd3, suggesting that the M2 marker genes are not directly controlled by Jmjd3 through histone modification. On the other hand, H3K27 trimethylation of transcription factors such as Irf4 and Cebpb was differentially regulated by wild-type and Jmjd3−/− macrophages. The expression of Irf4 was diminished in Jmjd3−/− macrophages, and its expression was restored
in a Jmjd3 demethylase-dependent manner. Indeed, Irf4−/− mice showed severe defects in M2 macrophage polarization in response to chitin administration and induction of BM macrophages in the presence of M-CSF. Although Jmjd3 also controls a set of transcription factors, Irf4 is one of the critical target genes responsible for controlling M2 macrophage polarization (Fig. 2). Differential involvement of IRF transcription factors can be important for M1 and M2 macrophage polarization. It was reported that IRF5 is involved in the differentiation of M1 macrophages, though it is currently unclear whether Irf5 is epigenetically controlled by histone modifications 41. Jmjd3 is specifically involved in M2 macrophage polarization without affecting M1, despite the fact that Jmjd3 is TLR-inducible in macrophages.