Fig. 3: OLZ and HFD promote hepatic lipid storage.

Frozen sections of liver were stained with Oil Red O as described in Materials and Methods (panel A, representative pictures) and staining was quantitated in all samples (panel B, left). Lipids (TG and NEFA) were extracted from pulverized liver samples and determined by colorimetric assay (panel B, right). Expression of key genes involved in de novo lipid genesis and catabolism were determined by real-time rtPCR (Panel B, right). ^aP <0.05 compared to LFD; ^bP <0.05 compared to absence of OLZ by 2-way ANOVA with Tukey’s post-hoc analysis.