scvelo
БесплатноЗапускает вложенные скриптыНе проверенRNA velocity analysis with scVelo. Estimate cell state transitions from unspliced/spliced mRNA dynamics, infer trajectory directions, compute latent time, and i
Об этом скилле
scVelo — RNA Velocity Analysis
Overview
scVelo is the leading Python package for RNA velocity analysis in single-cell RNA-seq data. It infers cell state transitions by modeling the kinetics of mRNA splicing — using the ratio of unspliced (pre-mRNA) to spliced (mature mRNA) abundances to determine whether a gene is being upregulated or downregulated in each cell. This allows reconstruction of developmental trajectories and identification of cell fate decisions without requiring time-course data.
Installation: pip install scvelo
Key resources:
- Documentation: https://scvelo.readthedocs.io/
- GitHub: https://github.com/theislab/scvelo
- Paper: Bergen et al. (2020) Nature Biotechnology. PMID: 32747759
When to Use This Skill
Use scVelo when:
- Trajectory inference from snapshot data: Determine which direction cells are differentiating
- Cell fate prediction: Identify progenitor cells and their downstream fates
- Driver gene identification: Find genes whose dynamics best explain observed trajectories
- Developmental biology: Model hematopoiesis, neurogenesis, epithelial-to-mesenchymal transitions
- Latent time estimation: Order cells along a pseudotime derived from splicing dynamics
- Complement to Scanpy: Add directional information to UMAP embeddings
Prerequisites
scVelo requires count matrices for both unspliced and spliced RNA. These are generated by:
- STARsolo or kallisto|bustools with
lamannomode - velocyto CLI:
velocyto run10x/velocyto run - alevin-fry / simpleaf with spliced/unspliced output
Data is stored in an AnnData object with layers["spliced"] and layers["unspliced"].
Standard RNA Velocity Workflow
1. Setup and Data Loading
import scvelo as scv
import scanpy as sc
import numpy as np
import matplotlib.pyplot as plt
# Configure settings
scv.settings.verbosity = 3 # Show computation steps
scv.settings.presenter_view = True
scv.settings.set_figure_params('scvelo')
# Load data (AnnData with spliced/unspliced layers)
# Option A: Load from loom (velocyto output)
adata = scv.read("cellranger_output.loom", cache=True)
# Option B: Merge velocyto loom with Scanpy-processed AnnData
adata_processed = sc.read_h5ad("processed.h5ad") # Has UMAP, clusters
adata_velocity = scv.read("velocyto.loom")
adata = scv.utils.merge(adata_processed, adata_velocity)
# Verify layers
print(adata)
# obs × var: N × G
# layers: 'spliced', 'unspliced' (required)
# obsm['X_umap'] (required for visualization)
2. Preprocessing
# Filter and normalize (follows Scanpy conventions)
scv.pp.filter_and_normalize(
adata,
min_shared_counts=20, # Minimum counts in spliced+unspliced
n_top_genes=2000 # Top highly variable genes
)
# Compute first and second order moments (means and variances)
# knn_connectivities must be computed first
sc.pp.neighbors(adata, n_neighbors=30, n_pcs=30)
scv.pp.moments(
adata,
n_pcs=30,
n_neighbors=30
)
3. Velocity Estimation — Stochastic Model
The stochastic model is fast and suitable for exploratory analysis:
# Stochastic velocity (faster, less accurate)
scv.tl.velocity(adata, mode='stochastic')
scv.tl.velocity_graph(adata)
# Visualize
scv.pl.velocity_embedding_stream(
adata,
basis='umap',
color='leiden',
title="RNA Velocity (Stochastic)"
)
4. Velocity Estimation — Dynamical Model (Recommended)
The dynamical model fits the full splicing kinetics and is more accurate:
# Recover dynamics (computationally intensive; ~10-30 min for 10K cells)
scv.tl.recover_dynamics(adata, n_jobs=4)
# Compute velocity from dynamical model
scv.tl.velocity(adata, mode='dynamical')
scv.tl.velocity_graph(adata)
5. Latent Time
The dynamical model enables computation of a shared latent time (pseudotime):
# Compute latent time
scv.tl.latent_time(adata)
# Visualize latent time on UMAP
scv.pl.scatter(
adata,
color='latent_time',
color_map='gnuplot',
size=80,
title='Latent time'
)
# Identify top genes ordered by latent time
top_genes = adata.var['fit_likelihood'].sort_values(ascending=False).index[:300]
scv.pl.heatmap(
adata,
var_names=top_genes,
sortby='latent_time',
col_color='leiden',
n_convolve=100
)
6. Driver Gene Analysis
# Identify genes with highest velocity fit
scv.tl.rank_velocity_genes(adata, groupby='leiden', min_corr=0.3)
df = scv.DataFrame(adata.uns['rank_velocity_genes']['names'])
print(df.head(10))
# Speed and coherence
scv.tl.velocity_confidence(adata)
scv.pl.scatter(
adata,
c=['velocity_length', 'velocity_confidence'],
cmap='coolwarm',
perc=[5, 95]
)
# Phase portraits for specific genes
scv.pl.velocity(adata, ['Cpe', 'Gnao1', 'Ins2'],
ncols=3, figsize=(16, 4))
7. Velocity Arrows and Pseudotime
# Arrow plot on UMAP
scv.pl.velocity_embedding(
adata,
arrow_length=3,
arrow_size=2,
color='leiden',
basis='umap'
)
# Stream plot (cleaner visualization)
scv.pl.velocity_embedding_stream(
adata,
basis='umap',
color='leiden',
smooth=0.8,
min_mass=4
)
# Velocity pseudotime (alternative to latent time)
scv.tl.velocity_pseudotime(adata)
scv.pl.scatter(adata, color='velocity_pseudotime', cmap='gnuplot')
8. PAGA Trajectory Graph
# PAGA graph with velocity-informed transitions
scv.tl.paga(adata, groups='leiden')
df = scv.get_df(adata, 'paga/transitions_confidence', precision=2).T
df.style.background_gradient(cmap='Blues').format('{:.2g}')
# Plot PAGA with velocity
scv.pl.paga(
adata,
basis='umap',
size=50,
alpha=0.1,
min_edge_width=2,
node_size_scale=1.5
)
Complete Workflow Script
import scvelo as scv
import scanpy as sc
def run_rna_velocity(adata, n_top_genes=2000, mode='dynamical', n_jobs=4):
"""
Complete RNA velocity workflow.
Args:
adata: AnnData with 'spliced' and 'unspliced' layers, UMAP in obsm
n_top_genes: Number of top HVGs for velocity
mode: 'stochastic' (fast) or 'dynamical' (accurate)
n_jobs: Parallel jobs for dynamical model
Returns:
Processed AnnData with velocity information
"""
scv.settings.verbosity = 2
# 1. Preprocessing
scv.pp.filter_and_normalize(adata, min_shared_counts=20, n_top_genes=n_top_genes)
if 'neighbors' not in adata.uns:
sc.pp.neighbors(adata, n_neighbors=30)
scv.pp.moments(adata, n_pcs=30, n_neighbors=30)
# 2. Velocity estimation
if mode == 'dynamical':
scv.tl.recover_dynamics(adata, n_jobs=n_jobs)
scv.tl.velocity(adata, mode=mode)
scv.tl.velocity_graph(adata)
# 3. Downstream analyses
if mode == 'dynamical':
scv.tl.latent_time(adata)
scv.tl.rank_velocity_genes(adata, groupby='leiden', min_corr=0.3)
scv.tl.velocity_confidence(adata)
scv.tl.velocity_pseudotime(adata)
return adata
Key Output Fields in AnnData
After running the workflow, the following fields are added:
| Location | Key | Description |
|---|---|---|
adata.layers |
velocity |
RNA velocity per gene per cell |
adata.layers |
fit_t |
Fitted latent time per gene per cell |
adata.obsm |
velocity_umap |
2D velocity vectors on UMAP |
adata.obs |
velocity_pseudotime |
Pseudotime from velocity |
adata.obs |
latent_time |
Latent time from dynamical model |
adata.obs |
velocity_length |
Speed of each cell |
adata.obs |
velocity_confidence |
Confidence score per cell |
adata.var |
fit_likelihood |
Gene-level model fit quality |
adata.var |
fit_alpha |
Transcription rate |
adata.var |
fit_beta |
Splicing rate |
adata.var |
fit_gamma |
Degradation rate |
adata.uns |
velocity_graph |
Cell-cell transition probability matrix |
Velocity Models Comparison
| Model | Speed | Acc
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FAQ
Что делает скилл scvelo?
RNA velocity analysis with scVelo. Estimate cell state transitions from unspliced/spliced mRNA dynamics, infer trajectory directions, compute latent time, and identify driver genes in single-cell RNA-seq data. Complements Scanpy/scVI-tools for trajectory inference.
Как установить скилл scvelo?
Скопируй папку скилла в ~/.claude/skills (вкладка Claude Code выше делает это одной командой), либо поставь как плагин.
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