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Repository scanpy_cluster_reduce_dimension
Owner: iuc
Synopsis: Wrapper for the scanpy tool suite: Scanpy cluster, embed
Scanpy is a scalable toolkit for analyzing single-cell gene expression data. It includes preprocessing, visualization, clustering, pseudotime and trajectory inference and differential expression testing.
Content homepage: https://scanpy.readthedocs.io
Type: unrestricted
Revision: 0:0e212e42ef88
This revision can be installed: True
Times cloned / installed: 974

Repository README files - may contain important installation or license information

The different methods from Scanpy have been grouped by themes: 1. Filter in `filter.xml` - Filter cell outliers based on counts and numbers of genes expressed, using `pp.filter_cells` - Filter genes based on number of cells or counts, using `pp.filter_genes` - Extract highly variable genes, using `pp.filter_genes_dispersion` - `tl.highly_variable_genes` (need to be added) - Subsample to a fraction of the number of observations, using `pp.subsample` - `queries.gene_coordinates` (need to be added) - `queries.mitochondrial_genes` (need to be added) 2. Normalize in `normalize.xml` - Normalize total counts per cell, using `pp.normalize_per_cell` - Normalization and filtering as of Zheng et al. (2017), using `pp.recipe_zheng17` - Normalization and filtering as of Weinreb et al (2017), using `pp.recipe_weinreb17` - Normalization and filtering as of Seurat et al (2015), using `pp.recipe_seurat` - Logarithmize the data matrix, using `pp.log1p` - Scale data to unit variance and zero mean, using `pp.scale` - Square root the data matrix, using `pp.sqrt` - Downsample counts, using `pp.downsample_counts` 3. Remove confounder in `remove_confounders.xml` - Regress out unwanted sources of variation, using `pp.regress_out` - `pp.mnn_correct` (need to be added) - `pp.mnn_correct` (need to be added) - `pp.magic` (need to be added) - `tl.sim` (need to be added) - `pp.calculate_qc_metrics` (need to be added) - Score a set of genes, using `tl.score_genes` - Score cell cycle genes, using `tl.score_genes_cell_cycle` - `tl.cyclone` (need to be added) - `tl.andbag` (need to be added) 4. Cluster and reduce dimension in `cluster_reduce_dimension.xml` - `tl.leiden` (need to be added) - Cluster cells into subgroups, using `tl.louvain` - Computes PCA (principal component analysis) coordinates, loadings and variance decomposition, using `pp.pca` - Computes PCA (principal component analysis) coordinates, loadings and variance decomposition, using `tl.pca` - Diffusion Maps, using `tl.diffmap` - t-distributed stochastic neighborhood embedding (tSNE), using `tl.tsne` - Embed the neighborhood graph using UMAP, using `tl.umap` - `tl.phate` (need to be added) - Compute a neighborhood graph of observations, using `pp.neighbors` - Rank genes for characterizing groups, using `tl.rank_genes_groups` 4. Inspect - `tl.paga_compare_paths` (need to be added) - `tl.paga_degrees` (need to be added) - `tl.paga_expression_entropies` (need to be added) - Generate cellular maps of differentiation manifolds with complex topologies, using `tl.paga` - Infer progression of cells through geodesic distance along the graph, using `tl.dpt` 5. Plot 1. Generic - Scatter plot along observations or variables axes, using `pl.scatter` - Heatmap of the expression values of set of genes, using `pl.heatmap` - Makes a dot plot of the expression values, using `pl.dotplot` - Violin plot, using `pl.violin` - `pl.stacked_violin` (need to be added) - Heatmap of the mean expression values per cluster, using `pl.matrixplot` - Hierarchically-clustered heatmap, using `pl.clustermap` - `pl.ranking` 2. Preprocessing - Plot the fraction of counts assigned to each gene over all cells, using `pl.highest_expr_genes` - Plot dispersions versus means for genes, using `pl.filter_genes_dispersion` - `pl.highly_variable_genes` (need to be added) - `pl.calculate_qc_metrics` (need to be added) 3. PCA - Scatter plot in PCA coordinates, using `pl.pca` - Rank genes according to contributions to PCs, using `pl.pca_loadings` - Scatter plot in PCA coordinates, using `pl.pca_variance_ratio` - Plot PCA results, using `pl.pca_overview` 4. Embeddings - Scatter plot in tSNE basis, using `pl.tsne` - Scatter plot in UMAP basis, using `pl.umap` - Scatter plot in Diffusion Map basis, using `pl.diffmap` - `pl.draw_graph` (need to be added) 5. Branching trajectories and pseudotime, clustering - Plot groups and pseudotime, using `pl.dpt_groups_pseudotime` - Heatmap of pseudotime series, using `pl.dpt_timeseries` - Plot the abstracted graph through thresholding low-connectivity edges, using `pl.paga` - `pl.paga_compare` (need to be added) - `pl.paga_path` (need to be added) 6. Marker genes: - Plot ranking of genes using dotplot plot, using `pl.rank_gene_groups` - `pl.rank_genes_groups_dotplot` (need to be added) - `pl.rank_genes_groups_heatmap` (need to be added) - `pl.rank_genes_groups_matrixplot` (need to be added) - `pl.rank_genes_groups_stacked_violin` (need to be added) - `pl.rank_genes_groups_violin` (need to be added) 7. Misc - `pl.phate` (need to be added) - `pl.matrix` (need to be added) - `pl.paga_adjacency` (need to be added) - `pl.timeseries` (need to be added) - `pl.timeseries_as_heatmap` (need to be added) - `pl.timeseries_subplot` (need to be added)

Contents of this repository

Name Description Version Minimum Galaxy Version
1.4+galaxy0 16.01

Categories
Single Cell - Tools for single cell analyses
Spatial Omics - Tools for spacial omics
Transcriptomics - Tools for use in the study of Transcriptomics.