AnnData

Overview

AnnData is a Python package for handling annotated data matrices, storing experimental measurements (X) alongside observation metadata (obs), variable metadata (var), and multi-dimensional annotations (obsm, varm, obsp, varp, uns). Originally designed for single-cell genomics through Scanpy, it now serves as a general-purpose framework for any annotated data requiring efficient storage, manipulation, and analysis.

When to Use This Skill

Use this skill when:

• Creating, reading, or writing AnnData objects
• Working with h5ad, zarr, or other genomics data formats
• Performing single-cell RNA-seq analysis
• Managing large datasets with sparse matrices or backed mode
• Concatenating multiple datasets or experimental batches
• Subsetting, filtering, or transforming annotated data
• Integrating with scanpy, scvi-tools, or other scverse ecosystem tools

Installation

Requires Python 3.11+ (anndata 0.11+ dropped 3.9). Current stable release: 0.12.x.

uv pip install anndata

# Lazy I/O and dask-backed operations
uv pip install "anndata[dask,lazy]"

# Development / docs (contributors)
uv pip install "anndata[dev,test,doc]"

Quick Start

Creating an AnnData object

import anndata as ad
import numpy as np
import pandas as pd

# Minimal creation
X = np.random.rand(100, 2000)  # 100 cells × 2000 genes
adata = ad.AnnData(X)

# With metadata
obs = pd.DataFrame({
    'cell_type': ['T cell', 'B cell'] * 50,
    'sample': ['A', 'B'] * 50
}, index=[f'cell_{i}' for i in range(100)])

var = pd.DataFrame({
    'gene_name': [f'Gene_{i}' for i in range(2000)]
}, index=[f'ENSG{i:05d}' for i in range(2000)])

adata = ad.AnnData(X=X, obs=obs, var=var)

Reading data

# Native formats (read_h5ad/read_zarr remain at top-level)
adata = ad.read_h5ad('data.h5ad')
adata = ad.read_h5ad('large_data.h5ad', backed='r')  # lazy load for large files
adata = ad.read_zarr('data.zarr')

# Other formats: prefer anndata.io (top-level imports are deprecated)
from anndata.io import read_csv, read_loom, read_mtx

adata = read_csv('data.csv')
adata = read_loom('data.loom')

# 10X Genomics: use scanpy (not anndata) — see scanpy skill
import scanpy as sc
adata = sc.read_10x_h5('filtered_feature_bc_matrix.h5')
adata = sc.read_10x_mtx('filtered_feature_bc_matrix/')

Writing data

# Write h5ad file
adata.write_h5ad('output.h5ad')

# Write with compression
adata.write_h5ad('output.h5ad', compression='gzip')

# Write other formats
adata.write_zarr('output.zarr')
adata.write_csvs('output_dir/')

Basic operations

# Subset by conditions
t_cells = adata[adata.obs['cell_type'] == 'T cell']

# Subset by indices
subset = adata[0:50, 0:100]

# Add metadata
adata.obs['quality_score'] = np.random.rand(adata.n_obs)
adata.var['highly_variable'] = np.random.rand(adata.n_vars) > 0.8

# Access dimensions
print(f"{adata.n_obs} observations × {adata.n_vars} variables")

Core Capabilities

1. Data Structure

Understand the AnnData object structure including X, obs, var, layers, obsm, varm, obsp, varp, uns, and raw components.

See: references/data_structure.md for comprehensive information on:

• Core components (X, obs, var, layers, obsm, varm, obsp, varp, uns, raw)
• Creating AnnData objects from various sources
• Accessing and manipulating data components
• Memory-efficient practices

2. Input/Output Operations

Read and write data in various formats with support for compression, backed mode, and cloud storage.

See: references/io_operations.md for details on:

• Native formats (h5ad, zarr)
• Alternative formats (CSV, MTX, Loom, 10X, Excel)
• Backed mode for large datasets
• Remote data access
• Format conversion
• Performance optimization

Common commands:

from anndata.io import read_mtx

# Read/write h5ad
adata = ad.read_h5ad('data.h5ad', backed='r')
adata.write_h5ad('output.h5ad', compression='gzip')

# 10X Genomics (via scanpy)
import scanpy as sc
adata = sc.read_10x_h5('filtered_feature_bc_matrix.h5')

# Read MTX format
adata = read_mtx('matrix.mtx').T

3. Concatenation

Combine multiple AnnData objects along observations or variables with flexible join strategies.

See: references/concatenation.md for comprehensive coverage of:

• Basic concatenation (axis=0 for observations, axis=1 for variables)
• Join types (inner, outer)
• Merge strategies (same, unique, first, only)
• Tracking data sources with labels
• Lazy concatenation (AnnCollection)
• On-disk concatenation for large datasets

Common commands:

# Concatenate observations (combine samples)
adata = ad.concat(
    [adata1, adata2, adata3],
    axis=0,
    join='inner',
    label='batch',
    keys=['batch1', 'batch2', 'batch3']
)

# Concatenate variables (combine modalities)
adata = ad.concat([adata_rna, adata_protein], axis=1)

# Lazy concatenation
from anndata.experimental import AnnCollection
collection = AnnCollection(
    ['data1.h5ad', 'data2.h5ad'],
    join_obs='outer',
    label='dataset'
)

4. Data Manipulation

Transform, subset, filter, and reorganize data efficiently.

See: references/manipulation.md for detailed guidance on:

• Subsetting (by indices, names, boolean masks, metadata conditions)
• Transposition
• Copying (full copies vs views)
• Renaming (observations, variables, categories)
• Type conversions (strings to categoricals, sparse/dense)
• Adding/removing data components
• Reordering
• Quality control filtering

Common commands:

# Subset by metadata
filtered = adata[adata.obs['quality_score'] > 0.8]
hv_genes = adata[:, adata.var['highly_variable']]

# Transpose
adata_T = adata.T

# Copy vs view
view = adata[0:100, :]  # View (lightweight reference)
copy = adata[0:100, :].copy()  # Independent copy

# Convert strings to categoricals
adata.strings_to_categoricals()

5. Best Practices

Follow recommended patterns for memory efficiency, performance, and reproducibility.

See: references/best_practices.md for guidelines on:

• Memory management (sparse matrices, categoricals, backed mode)
• Views vs copies
• Data storage optimization
• Performance optimization
• Working with raw data
• Metadata management
• Reproducibility
• Error handling
• Integration with other tools
• Common pitfalls and solutions

Key recommendations:

# Use sparse matrices for sparse data
from scipy.sparse import csr_matrix
adata.X = csr_matrix(adata.X)

# Convert strings to categoricals
adata.strings_to_categoricals()

# Use backed mode for large files
adata = ad.read_h5ad('large.h5ad', backed='r')

# Store raw before filtering
adata.raw = adata.copy()
adata = adata[:, adata.var['highly_variable']]

Integration with Scverse Ecosystem

AnnData serves as the foundational data structure for the scverse ecosystem:

Scanpy (Single-cell analysis)

import scanpy as sc

# Preprocessing
sc.pp.filter_cells(adata, min_genes=200)
sc.pp.normalize_total(adata, target_sum=1e4)
sc.pp.log1p(adata)
sc.pp.highly_variable_genes(adata, n_top_genes=2000)

# Dimensionality reduction
sc.pp.pca(adata, n_comps=50)
sc.pp.neighbors(adata, n_neighbors=15)
sc.tl.umap(adata)
sc.tl.leiden(adata)

# Visualization
sc.pl.umap(adata, color=['cell_type', 'leiden'])

Muon (Multimodal data)

import muon as mu

# Combine RNA and protein data
mdata = mu.MuData({'rna': adata_rna, 'protein': adata_protein})

PyTorch integration

from anndata.experimental import AnnLoader

# Create DataLoader for deep learning
dataloader = AnnLoader(adata, batch_size=128, shuffle=True)

for batch in dataloader:
    X = batch.X
    # Train model

Common Workflows

Single-cell RNA-seq analysis

import anndata as ad
import scanpy as sc

# 1. Load data (10X via scanpy; anndata handles h5ad/zarr natively)
adata = sc.read_10x_h5('filtered_feature_bc_matrix.h5')

# 2. Quality control
adata.obs['n_genes'] = (adata.X > 0).sum(axis=1)
adata.obs['n_counts'] = adata.X.sum(axis=1)
adata = adata[adata.obs['n_genes'] > 200]
adata = adata[adata.obs['n_counts'] < 50000]

# 3. Store raw
adata.raw = adata.copy()

# 4. Normalize and filter
sc.pp.normalize_total(adata, target_sum=1e4)
sc.pp.log1p(adata)
sc.pp.highly_variable_genes(adata, n_top_genes=2000)
adata = adata[:, adata.var['highly_variable']]

# 5. Save processed data
adata.write_h5ad('processed.h5ad')

Batch integration

# Load multiple batches
adata1 = ad.read_h5ad('batch1.h5ad')
adata2 = ad.read_h5ad('batch2.h5ad')
adata3 = ad.read_h5ad('batch3.h5ad')

# Concatenate with batch labels
adata = ad.concat(
    [adata1, adata2, adata3],
    label='batch',
    keys=['batch1', 'batch2', 'batch3'],
    join='inner'
)

# Apply batch correction
import scanpy as sc
sc.pp.combat(adata, key='batch')

# Continue analysis
sc.pp.pca(adata)
sc.pp.neighbors(adata)
sc.tl.umap(adata)

Working with large datasets

# Open in backed mode
adata = ad.read_h5ad('100GB_dataset.h5ad', backed='r')

# Filter based on metadata (no data loading)
high_quality = adata[adata.obs['quality_score'] > 0.8]

# Load filtered subset
adata_subset = high_quality.to_memory()

# Process subset
process(adata_subset)

# Or process in chunks
chunk_size = 1000
for i in range(0, adata.n_obs, chunk_size):
    chunk = adata[i:i+chunk_size, :].to_memory()
    process(chunk)

Troubleshooting

Out of memory errors

Use backed mode or convert to sparse matrices:

# Backed mode
adata = ad.read_h5ad('file.h5ad', backed='r')

# Sparse matrices
from scipy.sparse import csr_matrix
adata.X = csr_matrix(adata.X)

Slow file reading

Use compression and appropriate formats:

# Optimize for storage
adata.strings_to_categoricals()
adata.write_h5ad('file.h5ad', compression='gzip')

# Use Zarr for cloud storage (v3 optional since anndata 0.12)
import anndata
anndata.settings.zarr_write_format = 3  # default is 2
adata.write_zarr('file.zarr', chunks=(1000, 1000))

Index alignment issues

Always align external data on index:

# Wrong
adata.obs['new_col'] = external_data['values']

# Correct
adata.obs['new_col'] = external_data.set_index('cell_id').loc[adata.obs_names, 'values']

Additional Resources

• Official documentation: https://anndata.readthedocs.io/
• Scanpy tutorials: https://scanpy.readthedocs.io/
• Scverse ecosystem: https://scverse.org/
• GitHub repository: https://github.com/scverse/anndata