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Image Search Results
Journal: Nature Communications
Article Title: Long non-coding RNA Gm15441 attenuates hepatic inflammasome activation in response to PPARA agonism and fasting
doi: 10.1038/s41467-020-19554-7
Figure Lengend Snippet: a Venn diagrams of RefSeq transcripts and lncRNA transcripts that were differentially regulated by WY-14643 (fold change > 2 at FDR < 0.05) in wild-type and in Ppara −/− mouse liver, as determined by RNA-seq. 123 of the RefSeq genes are non-coding, indicated by their NR accession numbers. Six RefSeq genes and six lncRNA genes show opposite responses to WY-14643 treatment and are excluded from the gene counts shown. b Relative basal lncRNA expression in select tissues. c LncRNA expression in tissues from Ppara +/+ and Ppara −/− mice treated with WY-14643 for 48 h. At least five mice were analyzed for each genotype and treatment group. Each bar represents the mean ± SD for n = 5 tissue samples. Adjusted p values, provided in the panels, as determined by ANOVA with Tukey’s multiple comparison correction, one-sided for comparisons to Ppara +/+ mice or as shown (dashed horizontal lines). ND not detected.
Article Snippet: High quality RNA samples (RIN > 9.0) were pooled, as described below, and used to construct stranded RNA-seq libraries from polyA-selected total
Techniques: RNA Sequencing, Expressing, Comparison
Journal: Nature Communications
Article Title: Long non-coding RNA Gm15441 attenuates hepatic inflammasome activation in response to PPARA agonism and fasting
doi: 10.1038/s41467-020-19554-7
Figure Lengend Snippet: Wild-type ( Ppara +/+ ) mice were treated with WY-14643 and stranded RNA-seq was performed on total liver mRNA. a Expression of the antisense lncRNA Gm15441 is strongly upregulated. b Expression of the protein-coding Txnip mRNA is downregulated. Shown are the changes in expression of Gm15441 ( c ), and Txnip ( d ), mRNAs in Ppara +/+ and Ppara −/− mice treated with WY-14643, or vehicle control, for 48 h, determined by qRT-PCR. e Time course for changes in expression of Gm15441 and Txnip mRNA over a 24 h period following treatment with WY-14643 by gavage, determined by qRT-PCR. The maximum response of Txnip mRNA was seen at 1.5 h and for Gm15441 was seen at 6 h. Each data point represents the mean ± SD for n = 5 liver samples. Adjusted p values, provided in the panels, as determined by ANOVA with Tukey’s multiple comparison correction, two-sided for comparisons to Ppara +/+ mice or as shown (dashed horizontal line).
Article Snippet: High quality RNA samples (RIN > 9.0) were pooled, as described below, and used to construct stranded RNA-seq libraries from polyA-selected total
Techniques: RNA Sequencing, Expressing, Control, Quantitative RT-PCR, Comparison
Journal: Nature Communications
Article Title: Long non-coding RNA Gm15441 attenuates hepatic inflammasome activation in response to PPARA agonism and fasting
doi: 10.1038/s41467-020-19554-7
Figure Lengend Snippet: a Schematic representation of GFP construct inserts with or without the TXNIP 5′UTR sequence. b Analysis of Gm15441 RNA and Gfp mRNA in Hepa-1 cells. c Western blot analysis of GFP protein and relative density of GFP signal from Hepa-1 cells (right). d Fluorescence of GFP in Hepa-1 cells transfected with GFP with empty or Gm15441 plasmid DNA for 48 h ( n = 3). Scale bars represent 20 nm (100x). e Fluorescence of GFP in Hepa-1 cells transfected with 5′ UTR sequence containing GFP with empty or Gm15441 plasmid DNA for 48 h ( n = 3). Scale bars represent 20 nm (100x). f Analysis of Hfe2 , Pol3gl , and Ankrd34a mRNAs from Hepa-1 and NIHT3T cells transfected with empty plasmid or Gm15441 expression vector for 24 h. Each data point represents mean ± SD for n = 3 replicates. Adjusted p values, provided in the panels, as determined by ANOVA with Tukey’s multiple comparison correction, one-sided for comparisons in the absence of Gm15441 ( b , c ) or to empty vector ( f ). g Model for role of Gm15441 in suppressing TXNIP-mediated inflammasome activation.
Article Snippet: High quality RNA samples (RIN > 9.0) were pooled, as described below, and used to construct stranded RNA-seq libraries from polyA-selected total
Techniques: Construct, Sequencing, Western Blot, Fluorescence, Transfection, Plasmid Preparation, Expressing, Comparison, Activation Assay