Scanpy: Single-Cell Analysis
Overview
Scanpy is a scalable Python toolkit for analyzing single-cell RNA-seq data, built on AnnData. Apply this skill for complete single-cell workflows including quality control, normalization, dimensionality reduction, clustering, marker gene identification, visualization, and trajectory analysis.
When to Use This Skill
This skill should be used when:
- Analyzing single-cell RNA-seq data (.h5ad, 10X, CSV formats)
- Performing quality control on scRNA-seq datasets
- Creating UMAP, t-SNE, or PCA visualizations
- Identifying cell clusters and finding marker genes
- Annotating cell types based on gene expression
- Conducting trajectory inference or pseudotime analysis
- Generating publication-quality single-cell plots
Quick Start
Basic Import and Setup
import scanpy as sc import pandas as pd import numpy as np # Configure settings sc.settings.verbosity = 3 sc.settings.set_figure_params(dpi=80, facecolor='white') sc.settings.figdir = './figures/'
Loading Data
# From 10X Genomics adata = sc.read_10x_mtx('path/to/data/') adata = sc.read_10x_h5('path/to/data.h5') # From h5ad (AnnData format) adata = sc.read_h5ad('path/to/data.h5ad') # From CSV adata = sc.read_csv('path/to/data.csv')
Understanding AnnData Structure
The AnnData object is the core data structure in scanpy:
adata.X # Expression matrix (cells × genes) adata.obs # Cell metadata (DataFrame) adata.var # Gene metadata (DataFrame) adata.uns # Unstructured annotations (dict) adata.obsm # Multi-dimensional cell data (PCA, UMAP) adata.raw # Raw data backup # Access cell and gene names adata.obs_names # Cell barcodes adata.var_names # Gene names
Standard Analysis Workflow
1. Quality Control
Identify and filter low-quality cells and genes:
# Identify mitochondrial genes adata.var['mt'] = adata.var_names.str.startswith('MT-') # Calculate QC metrics sc.pp.calculate_qc_metrics(adata, qc_vars=['mt'], inplace=True) # Visualize QC metrics sc.pl.violin(adata, ['n_genes_by_counts', 'total_counts', 'pct_counts_mt'], jitter=0.4, multi_panel=True) # Filter cells and genes sc.pp.filter_cells(adata, min_genes=200) sc.pp.filter_genes(adata, min_cells=3) adata = adata[adata.obs.pct_counts_mt < 5, :] # Remove high MT% cells
Use the QC script for automated analysis:
python scripts/qc_analysis.py input_file.h5ad --output filtered.h5ad
2. Normalization and Preprocessing
# Normalize to 10,000 counts per cell sc.pp.normalize_total(adata, target_sum=1e4) # Log-transform sc.pp.log1p(adata) # Save raw counts for later adata.raw = adata # Identify highly variable genes sc.pp.highly_variable_genes(adata, n_top_genes=2000) sc.pl.highly_variable_genes(adata) # Subset to highly variable genes adata = adata[:, adata.var.highly_variable] # Regress out unwanted variation sc.pp.regress_out(adata, ['total_counts', 'pct_counts_mt']) # Scale data sc.pp.scale(adata, max_value=10)
3. Dimensionality Reduction
# PCA sc.tl.pca(adata, svd_solver='arpack') sc.pl.pca_variance_ratio(adata, log=True) # Check elbow plot # Compute neighborhood graph sc.pp.neighbors(adata, n_neighbors=10, n_pcs=40) # UMAP for visualization sc.tl.umap(adata) sc.pl.umap(adata, color='leiden') # Alternative: t-SNE sc.tl.tsne(adata)
4. Clustering
# Leiden clustering (recommended) sc.tl.leiden(adata, resolution=0.5) sc.pl.umap(adata, color='leiden', legend_loc='on data') # Try multiple resolutions to find optimal granularity for res in [0.3, 0.5, 0.8, 1.0]: sc.tl.leiden(adata, resolution=res, key_added=f'leiden_{res}')
5. Marker Gene Identification
# Find marker genes for each cluster sc.tl.rank_genes_groups(adata, 'leiden', method='wilcoxon') # Visualize results sc.pl.rank_genes_groups(adata, n_genes=25, sharey=False) sc.pl.rank_genes_groups_heatmap(adata, n_genes=10) sc.pl.rank_genes_groups_dotplot(adata, n_genes=5) # Get results as DataFrame markers = sc.get.rank_genes_groups_df(adata, group='0')
6. Cell Type Annotation
# Define marker genes for known cell types marker_genes = ['CD3D', 'CD14', 'MS4A1', 'NKG7', 'FCGR3A'] # Visualize markers sc.pl.umap(adata, color=marker_genes, use_raw=True) sc.pl.dotplot(adata, var_names=marker_genes, groupby='leiden') # Manual annotation cluster_to_celltype = { '0': 'CD4 T cells', '1': 'CD14+ Monocytes', '2': 'B cells', '3': 'CD8 T cells', } adata.obs['cell_type'] = adata.obs['leiden'].map(cluster_to_celltype) # Visualize annotated types sc.pl.umap(adata, color='cell_type', legend_loc='on data')
7. Save Results
# Save processed data adata.write('results/processed_data.h5ad') # Export metadata adata.obs.to_csv('results/cell_metadata.csv') adata.var.to_csv('results/gene_metadata.csv')
Common Tasks
Creating Publication-Quality Plots
# Set high-quality defaults sc.settings.set_figure_params(dpi=300, frameon=False, figsize=(5, 5)) sc.settings.file_format_figs = 'pdf' # UMAP with custom styling sc.pl.umap(adata, color='cell_type', palette='Set2', legend_loc='on data', legend_fontsize=12, legend_fontoutline=2, frameon=False, save='_publication.pdf') # Heatmap of marker genes sc.pl.heatmap(adata, var_names=genes, groupby='cell_type', swap_axes=True, show_gene_labels=True, save='_markers.pdf') # Dot plot sc.pl.dotplot(adata, var_names=genes, groupby='cell_type', save='_dotplot.pdf')
Refer to references/plotting_guide.md for comprehensive visualization examples.
Trajectory Inference
# PAGA (Partition-based graph abstraction) sc.tl.paga(adata, groups='leiden') sc.pl.paga(adata, color='leiden') # Diffusion pseudotime adata.uns['iroot'] = np.flatnonzero(adata.obs['leiden'] == '0')[0] sc.tl.dpt(adata) sc.pl.umap(adata, color='dpt_pseudotime')
Differential Expression Between Conditions
# Compare treated vs control within cell types adata_subset = adata[adata.obs['cell_type'] == 'T cells'] sc.tl.rank_genes_groups(adata_subset, groupby='condition', groups=['treated'], reference='control') sc.pl.rank_genes_groups(adata_subset, groups=['treated'])
Gene Set Scoring
# Score cells for gene set expression gene_set = ['CD3D', 'CD3E', 'CD3G'] sc.tl.score_genes(adata, gene_set, score_name='T_cell_score') sc.pl.umap(adata, color='T_cell_score')
Batch Correction
# ComBat batch correction sc.pp.combat(adata, key='batch') # Alternative: use Harmony or scVI (separate packages)
Key Parameters to Adjust
Quality Control
min_genes: Minimum genes per cell (typically 200-500)min_cells: Minimum cells per gene (typically 3-10)pct_counts_mt: Mitochondrial threshold (typically 5-20%)
Normalization
target_sum: Target counts per cell (default 1e4)
Feature Selection
n_top_genes: Number of HVGs (typically 2000-3000)min_mean,max_mean,min_disp: HVG selection parameters
Dimensionality Reduction
n_pcs: Number of principal components (check variance ratio plot)n_neighbors: Number of neighbors (typically 10-30)
Clustering
resolution: Clustering granularity (0.4-1.2, higher = more clusters)
Common Pitfalls and Best Practices
- Always save raw counts:
adata.raw = adatabefore filtering genes - Check QC plots carefully: Adjust thresholds based on dataset quality
- Use Leiden over Louvain: More efficient and better results
- Try multiple clustering resolutions: Find optimal granularity
- Validate cell type annotations: Use multiple marker genes
- Use
use_raw=Truefor gene expression plots: Shows original counts - Check PCA variance ratio: Determine optimal number of PCs
- Save intermediate results: Long workflows can fail partway through
Bundled Resources
scripts/qc_analysis.py
Automated quality control script that calculates metrics, generates plots, and filters data:
python scripts/qc_analysis.py input.h5ad --output filtered.h5ad \ --mt-threshold 5 --min-genes 200 --min-cells 3
references/standard_workflow.md
Complete step-by-step workflow with detailed explanations and code examples for:
- Data loading and setup
- Quality control with visualization
- Normalization and scaling
- Feature selection
- Dimensionality reduction (PCA, UMAP, t-SNE)
- Clustering (Leiden, Louvain)
- Marker gene identification
- Cell type annotation
- Trajectory inference
- Differential expression
Read this reference when performing a complete analysis from scratch.
references/api_reference.md
Quick reference guide for scanpy functions organized by module:
- Reading/writing data (
sc.read_*,adata.write_*) - Preprocessing (
sc.pp.*) - Tools (
sc.tl.*) - Plotting (
sc.pl.*) - AnnData structure and manipulation
- Settings and utilities
Use this for quick lookup of function signatures and common parameters.
references/plotting_guide.md
Comprehensive visualization guide including:
- Quality control plots
- Dimensionality reduction visualizations
- Clustering visualizations
- Marker gene plots (heatmaps, dot plots, violin plots)
- Trajectory and pseudotime plots
- Publication-quality customization
- Multi-panel figures
- Color palettes and styling
Consult this when creating publication-ready figures.
assets/analysis_template.py
Complete analysis template providing a full workflow from data loading through cell type annotation. Copy and customize this template for new analyses:
cp assets/analysis_template.py my_analysis.py # Edit parameters and run python my_analysis.py
The template includes all standard steps with configurable parameters and helpful comments.
Additional Resources
- Official scanpy documentation: https://scanpy.readthedocs.io/
- Scanpy tutorials: https://scanpy-tutorials.readthedocs.io/
- scverse ecosystem: https://scverse.org/ (related tools: squidpy, scvi-tools, cellrank)
- Best practices: Luecken & Theis (2019) "Current best practices in single-cell RNA-seq"
Tips for Effective Analysis
- Start with the template: Use
assets/analysis_template.pyas a starting point - Run QC script first: Use
scripts/qc_analysis.pyfor initial filtering - Consult references as needed: Load workflow and API references into context
- Iterate on clustering: Try multiple resolutions and visualization methods
- Validate biologically: Check marker genes match expected cell types
- Document parameters: Record QC thresholds and analysis settings
- Save checkpoints: Write intermediate results at key steps