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CapitalBio Corporation
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NimbleGen Systems GmbH
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imaGenes GmbH
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DataScience LTD
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Image Search Results
Journal: Blood
Article Title: p16 INK4a deficiency promotes IL-4-induced polarization and inhibits proinflammatory signaling in macrophages
doi: 10.1182/blood-2010-10-313106
Figure Lengend Snippet: Microarray analysis using mRNA from p16−/− BMDM compared to p16+/+ BMDM showed (A) decreased mRNA expression of classically activated macrophages-associated genes and (B) increased mRNA expression of alternatively activated macrophages-associated genes. Data is expressed as fold change relative to p16+/+ BMDM. (C) Differential gene expression in p16−/− BMDM relative to p16+/+ BMDM was correlated with the changes induced in IL-4-induced p16+/+ AAMφ. The figure shows 2log values of the probesets significantly (p<0.05) regulated only in p16−/− BMDM (red dots), only in IL-4-polarized p16+/+ AAMφ (green dots) and by both conditions (blue dots), compared to p16+/+ BMDM. The X-axis represents differences in gene expression induced by IL-4, whereas the Y-axis represents the effect of p16INKa-deficiency. These comparisons are depicted in the schematic representation of the protocol in the corresponding colors. Pearson Correlation analysis was done for probesets differentially expressed by both conditions (blue). (D) Heat map of p16+/+ BMDM, p16−/− BMDM, IL-4-polarized p16+/+ and p16−/− AAMφ gene expression profiles. Colors fluctuate from blue (poorly expressed) to green (intermediate expression) and yellow (high expression). Additional information regarding gene description, fold induction, and p-value can be found in Table S3.
Article Snippet: We thank E. Vallez for mouse breeding, J. Brozek (
Techniques: Microarray, Expressing, Gene Expression
Journal: Blood
Article Title: p16 INK4a deficiency promotes IL-4-induced polarization and inhibits proinflammatory signaling in macrophages
doi: 10.1182/blood-2010-10-313106
Figure Lengend Snippet: Representation of the relative microarray intensity values from a selection of down-regulated genes in p16+/+ and p16−/− BMDM with or without polarization (AAMφ) by 15 ng/mL IL-4 from day 0 of differentiation. Statistically significant differences are indicated (a: p<0.05 compared to p16+/+ BMDM; b: p<0.05 compared to p16−/− BMDM; c: p<0.05 compared to p16+/+ AAMφ.)
Article Snippet: We thank E. Vallez for mouse breeding, J. Brozek (
Techniques: Microarray, Selection
Journal: BMC Ophthalmology
Article Title: MiRNAs regulate oxidative stress related genes via binding to the 3′ UTR and TATA-box regions: a new hypothesis for cataract pathogenesis
doi: 10.1186/s12886-017-0537-9
Figure Lengend Snippet: Heatmap shows differentially expressed mRNAs in cataractous lens samples compared with transparent lens samples. Six separate microarray assays were performed to determine the genome-wide mRNA expression in the central epithelium of transparent and cataractous human lenses. Microarray data were processed by CapitalBio Corporation. Heatmap shows differentially expressed mRNAs in cataractous lens samples compared with transparent lens samples. Relative expression value from high to low was shown by gradient of red to green in the heatmap. Colors indicate relative mRNA expression. Red and green indicate higher or lower expression of mRNAs relative to those in transparent lens samples, respectively. FDR (false discovery rate) adjusted p -value <0.05
Article Snippet:
Techniques: Microarray, Genome Wide, Expressing
Journal: Toxicological Sciences
Article Title: Chronic Hexavalent Chromium Exposure Upregulates the RNA Methyltransferase METTL3 Expression to Promote Cell Transformation, Cancer Stem Cell-Like Property, and Tumorigenesis
doi: 10.1093/toxsci/kfac023
Figure Lengend Snippet: Total RNA N6-methyladenosine (m6A) modification levels are significantly increased in chronic hexavalent chromium [Cr(VI)] exposure-transformed human bronchial epithelial cells and chronic chromate-exposed mouse lung tissues. A, The heatmap from m6A microarray analysis showing the extent of total messenger RNA m6A methylation in passage-matched control cells (BEAS-2B-Control) and chronic Cr(VI) exposure-transformed cells [BEAS-2B-Cr(VI)]. B and C, Relative total RNA m6A levels measured by using the EpiQuik m6A RNA Methylation Quantification Kit. The total RNA m6A levels in Cr(VI)-transformed cells (B) or chromate-exposed mouse lung tissues (C) are expressed relative to the passage-matched control cells (means ± SD, n = 3) (B) or vehicle control-exposed mouse lungs (means ± SD, n = 6) (C), respectively. *p < .05.
Article Snippet: The
Techniques: Modification, Transformation Assay, Microarray, Methylation, Control
Journal: British Journal of Nutrition
Article Title: Peripheral blood mononuclear cell gene expression profile in obese boys who followed a moderate energy-restricted diet: differences between high and low responders at baseline and after the intervention
doi: 10.1017/s0007114514003584
Figure Lengend Snippet: Fig. 2. Heat map analysis of microarray data showing (a) hierarchical clustering of fifty-five differentially expressed genes between the low-responder (LR) group and the high-responder (HR) group at baseline (LB and HB, respectively), and (b) hierarchical clustering of forty-two differentially expressed genes in the HR group before (HB) and after (HA) the 10-week nutritional intervention programme. The red or green colours indicate differentially up- or down-regulated genes, respectively (1·5-fold change, P,0·05), in the samples from twelve obese boys from the two groups (HR and LR), (b) before and (a) after the intervention. The comparison of (a) HB v. LB and (b) HA v. HB is shown. For a list of gene names and abbreviations, see online supplementary Table S1. (A colour version of this figure can be found online at http://www.journals.cambridge.org/bjn).
Article Snippet: For the analysis,
Techniques: Microarray, Comparison