Promoter regulation in the COX-2 promoter-flanking region (−95∼−9

Promoter regulation in the COX-2 promoter-flanking region (−95∼−90) containing the cis-acting elements C/EBP DNA binding activity in silico was predicted in the laboratory. Notably, the C/EBP-α-regulated protein COX-2 showed a similar result to that observed in IL-13-treated conditions. The COX-1 protein was considered a constitutive isoform, equally expressed in almost all tissues, which did not have any effects. In contrast, a previous report demonstrated that this website IL-13 downregulates PPAR-γ/HO-1

via ER stress-stimulated calpain activation. Further examining the regulatory role of C/EBP-β in the expression of protective PPAR-γ and HO-1 signaling, we found that IL-13 regulated LPS-induced protein expression in a dose-dependent manner (Supporting Information Fig. 1). The data showed that IL-13 markedly decreased the induction of C/EBP-β and PPAR-γ/HO-1 expression by activated microglia cells, indicating that IL-13 reciprocally beta-catenin assay regulated C/EBP-α and C/EBP-β in activated microglia. Calpain has been demonstrated to be involved in ER stress-induced activated microglia cell death [5]. Further investigating the possible mechanisms of IL-13 regulation of calpain in association with C/EBP-β, PPAR-γ, and HO-1, the results showed that IL-13 markedly enhanced calpain-II protein expression (Fig. 3A) and activity (Fig. 3B(i)) in primary

activated microglia, but markedly reduced the functional activity of calpain inhibitors ALLN, ALLM, and Z-Leu-Leu-CHO (Fig. 3B(ii)). In terms of the role of calpain-II in IL-13-induced C/EBP-β, PPAR-γ, and HO-1 downregulation, calpain-II was shown to interact with C/EBP-β and PPAR-γ but not HO-1 with co-immunoprecipitation and Western blot in activated microglia. Calpain-II was specifically associated with C/EBP-β and PPAR-γ in activated BV-2 microglia cells with the presence of IL-13-treated cells compared with the IgG control (Fig. 3C). There was no direct interaction Org 27569 of HO-1 with calpain-II. To clarify if calpain cleaved C/EBP-β and PPAR-γ, C/EBP-β or PPAR-γ

were digested with recombinant calpain-II under various conditions in vitro cleavage assay. The incubation of C/EBP-β or PPAR-γ with recombinant m-calpain led to the complete digestion of C/EBP-β or PPAR-γ, as determined by Western blotting analysis (Fig. 3D). Moreover, the calpain inhibitor, Z-Leu-Leu-CHO, effectively reversed the IL-13-enhanced LPS-induced C/EBP-β downregulation, but not C/EBP-α and COX-2, in BV-2 microglia (Fig. 3E). These results indicated that calpain-II induction plays an important role in IL-13-triggered reduction of C/EBP-β and PPAR-γ in inflammation-activated microglia. Death of activated microglia could act as an endogenous mechanism for the resolution of brain inflammation [6]. Thus, the effect of knockdown of C/EBP-α expression was investigated to determine if C/EBP-α abolishes IL-13-enhanced apoptosis in activated microglia.

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