2D). Overt inflammation, as observed by H&E staining, was evident at 7 days after tamoxifen treatment (Supporting Fig. 2A). To assess the influence of HIF-dependent pathways this website on inflammatory gene expression in the liver, mice with a double disruption of Vhl and Hif-1α or Hif-2α were generated. The double disruption of Vhl and Hif-2α (VhlF/FHif2aF/F;AlbERcre+tamoxifen) ameliorated the increase in Il-6 and Il-1β, compared to littermate controls (VhlF/FHif2aF/F+tamoxifen) (Fig.

2E). In contrast, a significant increase in Il-6 and Il-1β gene expression was observed in mice with a double disruption of Vhl and Hif-1α, compared to littermate controls (Supporting Fig. 2B). Furthermore, 2 weeks after the loss of Vhl, a dramatic increase in liver lipid accumulation was observed by oil red O staining (Fig. 3A,B). The increase in lipid accumulation could be observed as early as 24 hours after Vhl disruption (Fig. 3C,D). The

compound disruption of Vhl and Hif-1α or Hif-2α demonstrated that the increase in lipid accumulation was caused by HIF-2α, but not HIF-1α (Fig. 3E,F). Consistent with oil red O staining, hepatic triglycerides and cholesterol increased after disruption of Vhl for 2 weeks (Fig. 3G). Together, these data demonstrate that HIF-2α is a direct regulator of liver inflammation and lipid accumulation in the liver. To understand the critical genes regulated after Vhl disruption, gene expression profiles of VhlF/F and VhlF/F;AlbERcre were assessed in livers isolated 24 hours or 2 weeks after Vhl click here disruption. In total, 3597 significantly regulated changes were identified after 2 weeks of Vhl deletion, whereas 470 genes were identified 24 hours after Vhl disruption (Fig. 4A; the full gene list with an average change of 1.5-fold is in Supporting Tables 2 and 3). The data suggested

that a rapid increase in genes critical for lipid synthesis was followed by an increase in genes important for fatty acid uptake. Consistent with the microarray data, an increase was observed in the expression of fatty acid synthase (Fasn) and sterol regulatory element binding factor-1C (Srebp-1c) at 3 days after Vhl disruption. Interestingly, at 14 days after Vhl disruption, a significant repression of Fasn and Srebp-1c was observed (Fig. 4B), whereas a rapid repression of Cd36 selleck screening library gene expression was observed after 3 days of Vhl disruption, followed by a dramatic increase in gene expression 14 days after the loss of Vhl (Fig. 4B). In addition, a significant decrease was observed in genes critical in fatty acid β-oxidation, and a decrease in carnitine palmitoyltransferase 1A (Cpt1a), carnitine palmitoyltransferase 2 (Cpt2), acyl-CoA oxidase 1 (Acox), and peroxisome proliferator-activated receptor alpha (Pparα) were observed after 2 weeks of Vhl disruption; Pparα expression did not reach statistical significance (Fig. 4C).