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Table 1 ) were normalized against the mean of the healthy control taken along within the same experiment and converted to percentages. Statistics were calculated using Welsch’s t test. The black line indicates the median value, the lower and upper hinges correspond to the 25th and 75th percentiles. The upper and lower whisker extend to 1.5∗IQR. (C) Showing the UMAP plots from Journal: iScience
Article Title: Imaging flow cytometry reveals divergent mitochondrial phenotypes in mitochondrial disease patients
doi: 10.1016/j.isci.2024.111496
Figure Lengend Snippet: Correlation of IFC features with phenotypic features (A) Correlation plot showing the correlation between IFC features and clinical phenotypes. All clinical features were converted to binary parameters (Yes = Present, No=Not present) and correlation was calculated using Spearman’s correlation. The color coding and dot size correlate with Spearman’s rho coefficient. (B) All significant correlations have been plotted as a boxplot. For the boxplots, the values of each of the five features (
Article Snippet: All graphs and
Techniques: Control, Whisker Assay
Journal: Scientific Reports
Article Title: Derivation of human primary prostate epithelial cell lines by differentially targeting the CDKN2A locus along with expression of hTERT
doi: 10.1038/s41598-024-71306-5
Figure Lengend Snippet: RNA-Seq Analysis showing gene expression and clustering of the immortalized cell lines and PrECs. ( a ) Principal Component Analysis (PCA) of the RNA-Seq data for all the clones and PrEC. ( b ) Prostate tissue UMAP plots obtained using scRNA-Seq by the Human Protein Atlas (with superimposed expression of Actin (ACTG1)) identify all distinct populations in the primary human prostate . ( c ) Gene expression heat map of predicted correlation scores (Preds) of each clone and hPrECs to the cell populations identified in the human prostate using scRNA-Seq. Prediction scores range from 0.0 to 1.0 (blue to dark red scale on the left). The distinct cell populations identified by the Human Atlas using single cell-RNA-Seq are labeled by color and a number (top of the heatmap and legend on the right). Clones and PrEC RNA-Seq samples were analyzed in triplicate. The prediction score in B indicate that the clones are most closely related to the basal prostatic population designated c2 (labeled red/orange in the first column of the heat map).
Article Snippet: Also, to establish what distinct cell populations were present in the parental PrECs, we used tools from the
Techniques: RNA Sequencing, Gene Expression, Clone Assay, Expressing, Labeling
Journal: Scientific Reports
Article Title: Derivation of human primary prostate epithelial cell lines by differentially targeting the CDKN2A locus along with expression of hTERT
doi: 10.1038/s41598-024-71306-5
Figure Lengend Snippet: RNA-Seq Analysis showing gene expression and clustering of the immortalized cell lines and PrECs. ( a ) Principal Component Analysis (PCA) of the RNA-Seq data for all the clones and PrEC. ( b ) Prostate tissue UMAP plots obtained using scRNA-Seq by the Human Protein Atlas (with superimposed expression of Actin (ACTG1)) identify all distinct populations in the primary human prostate . ( c ) Gene expression heat map of predicted correlation scores (Preds) of each clone and hPrECs to the cell populations identified in the human prostate using scRNA-Seq. Prediction scores range from 0.0 to 1.0 (blue to dark red scale on the left). The distinct cell populations identified by the Human Atlas using single cell-RNA-Seq are labeled by color and a number (top of the heatmap and legend on the right). Clones and PrEC RNA-Seq samples were analyzed in triplicate. The prediction score in B indicate that the clones are most closely related to the basal prostatic population designated c2 (labeled red/orange in the first column of the heat map).
Article Snippet: Fig. 6 RNA-Seq Analysis showing gene expression and clustering of the immortalized cell lines and PrECs. ( a ) Principal Component Analysis (PCA) of the RNA-Seq data for all the clones and PrEC. ( b )
Techniques: RNA Sequencing, Gene Expression, Clone Assay, Expressing, Labeling