mouse olfactory bulb st data Search Results


mouse olfactory bulb st data  (Spatial Transcriptomics Inc)
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Spatial Transcriptomics Inc mouse olfactory bulb st data
Analysis of <t>mouse</t> <t>olfactory</t> <t>bulb</t> <t>data.</t> a) H&E staining of the olfactory bulb (top) and the deconvolution results of all candidate methods displayed by the spatial scatter pie plot of cell‐type composition on each spatial location. The examined cell types were granule cells (GC), olfactory sensory neurons (OSNs), periglomerular cells (PGC), mitral/tufted cells (M‐TC), and external plexiform layer interneurons (EPL‐IN) b) Manual annotation of anatomic layers (top), including the granule cell layer (GCL), the mitral cell layer (MCL), the glomerular layer (GL), and the nerve layer (ONL), and the spatial domains of different deconvolution methods visualized by spatial scatters of specific domain types. c) Performance comparison between candidate deconvolution methods, including QR‐SIDE, STdeconvolve, CARDfree, RCTD, CARD, SPOTlight, and spatialDWLS in terms of NMI (left) and ARI (right). d) UMAP plots of gene expression for Topic 1, 2, 3 identified by QR‐SIDE. The color scheme of each topic domain was the same as in (b). e) The heatmap of normalized expression level for the top 10 DE genes for topic domain 1, 2, 3. f) The correlation between DE genes of identified domains and marker genes of each cell type. g) The mean expression level of an example marker gene list for QR‐SIDE, where Tyro3 was included as the interference marker gene of cell type GC. h) Left and middle panels: The estimated spot‐separable η scores of correct marker Penk and misclassified marker Tyro3 . Right panel: The line plots of mean η of all markers across all spatial spots and the RMSE between estimated cell‐type composition by varying the inclusion of top 3‐7 marker genes of each cell type as the input gene list and the deconvolution results using high‐quality marker genes (as shown in a).
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Analysis of mouse olfactory bulb data. a) H&E staining of the olfactory bulb (top) and the deconvolution results of all candidate methods displayed by the spatial scatter pie plot of cell‐type composition on each spatial location. The examined cell types were granule cells (GC), olfactory sensory neurons (OSNs), periglomerular cells (PGC), mitral/tufted cells (M‐TC), and external plexiform layer interneurons (EPL‐IN) b) Manual annotation of anatomic layers (top), including the granule cell layer (GCL), the mitral cell layer (MCL), the glomerular layer (GL), and the nerve layer (ONL), and the spatial domains of different deconvolution methods visualized by spatial scatters of specific domain types. c) Performance comparison between candidate deconvolution methods, including QR‐SIDE, STdeconvolve, CARDfree, RCTD, CARD, SPOTlight, and spatialDWLS in terms of NMI (left) and ARI (right). d) UMAP plots of gene expression for Topic 1, 2, 3 identified by QR‐SIDE. The color scheme of each topic domain was the same as in (b). e) The heatmap of normalized expression level for the top 10 DE genes for topic domain 1, 2, 3. f) The correlation between DE genes of identified domains and marker genes of each cell type. g) The mean expression level of an example marker gene list for QR‐SIDE, where Tyro3 was included as the interference marker gene of cell type GC. h) Left and middle panels: The estimated spot‐separable η scores of correct marker Penk and misclassified marker Tyro3 . Right panel: The line plots of mean η of all markers across all spatial spots and the RMSE between estimated cell‐type composition by varying the inclusion of top 3‐7 marker genes of each cell type as the input gene list and the deconvolution results using high‐quality marker genes (as shown in a).

Journal: Small Methods

Article Title: Robust Spatial Cell‐Type Deconvolution with Qualitative Reference for Spatial Transcriptomics

doi: 10.1002/smtd.202401145

Figure Lengend Snippet: Analysis of mouse olfactory bulb data. a) H&E staining of the olfactory bulb (top) and the deconvolution results of all candidate methods displayed by the spatial scatter pie plot of cell‐type composition on each spatial location. The examined cell types were granule cells (GC), olfactory sensory neurons (OSNs), periglomerular cells (PGC), mitral/tufted cells (M‐TC), and external plexiform layer interneurons (EPL‐IN) b) Manual annotation of anatomic layers (top), including the granule cell layer (GCL), the mitral cell layer (MCL), the glomerular layer (GL), and the nerve layer (ONL), and the spatial domains of different deconvolution methods visualized by spatial scatters of specific domain types. c) Performance comparison between candidate deconvolution methods, including QR‐SIDE, STdeconvolve, CARDfree, RCTD, CARD, SPOTlight, and spatialDWLS in terms of NMI (left) and ARI (right). d) UMAP plots of gene expression for Topic 1, 2, 3 identified by QR‐SIDE. The color scheme of each topic domain was the same as in (b). e) The heatmap of normalized expression level for the top 10 DE genes for topic domain 1, 2, 3. f) The correlation between DE genes of identified domains and marker genes of each cell type. g) The mean expression level of an example marker gene list for QR‐SIDE, where Tyro3 was included as the interference marker gene of cell type GC. h) Left and middle panels: The estimated spot‐separable η scores of correct marker Penk and misclassified marker Tyro3 . Right panel: The line plots of mean η of all markers across all spatial spots and the RMSE between estimated cell‐type composition by varying the inclusion of top 3‐7 marker genes of each cell type as the input gene list and the deconvolution results using high‐quality marker genes (as shown in a).

Article Snippet: These include the mouse olfactory bulb ST data from Spatial Transcriptomics v1.0 ( https://www.spatialresearch.org ), the four human hepatocellular carcinoma Visium datasets ( https://www.ncbi.nlm.nih.gov/sra?linkname=bioproject_sra_all&from_uid=858545 ), mouse anterior brain 10x Visium data ( https://support.10xgenomics.com/spatial‐gene‐expression/datasets/1.0.0/V1_Mouse_Brain_Sagittal_Anterior ), and mouse posterior brain 10x Visium data ( https://support.10xgenomics.com/spatial‐gene‐expression/datasets/1.0.0/V1_Mouse_Brain_Sagittal_Posterior ).

Techniques: Staining, Comparison, Gene Expression, Expressing, Marker