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alterlab-scvelo

@alterlab-ieu · 收录于 1 周前

Run RNA velocity analysis with scVelo on single-cell RNA-seq data — estimate cell-state transitions from spliced/unspliced mRNA dynamics, infer trajectory direction, compute latent time, and identify driver genes. Use when adding directionality to trajectories or studying differentiation dynamics from spliced/unspliced layers (velocyto/STARsolo output); for the general QC, clustering, UMAP, and differential-expression analysis pipeline prefer alterlab-scanpy instead, and for .h5ad data-structure I/O and layer wrangling prefer alterlab-anndata instead. Part of the AlterLab Academic Skills suite.

适合你,如果正在研究细胞分化动态或需要为单细胞轨迹添加方向性

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怎么用

技能原文 SKILL.md作者撰写 · MIT · a0064fd

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: uv pip install "scvelo==0.3.4" (latest as of mid-2025). Gotcha: scVelo's deps declare numpy>=1.17 with no upper bound, but the stack breaks under numpy 2.x — if you hit cryptic np.float_/dtype errors on import or in plotting, pin numpy<2 (e.g. numpy==1.26.4). pandas 2.x is fine on 0.3.x.

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:

  1. STARsolo or kallisto|bustools with lamanno mode
  2. velocyto CLI: velocyto run10x / velocyto run
  3. 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).
# scv.pp.moments runs PCA + a kNN graph internally if they're absent, so
# you do NOT need a separate sc.pp.neighbors call here. Calling moments with
# n_pcs/n_neighbors and ALSO running sc.pp.neighbors first just recomputes the
# graph with possibly mismatched params — let moments own it on a fresh object.
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 | Accuracy | When to Use | |-------|-------|----------|-------------| | stochastic | Fast | Moderate | Exploratory; large datasets | | deterministic | Medium | Moderate | Simple linear kinetics | | dynamical | Slow | High | Publication-quality; identifies driver genes |

Best Practices
  • Start with stochastic mode for exploration; switch to dynamical for final analysis
  • Need good coverage of unspliced reads: Short reads (< 100 bp) may miss intron coverage
  • Minimum 2,000 cells: RNA velocity is noisy with fewer cells
  • Velocity should be coherent: Arrows should follow known biology; randomness indicates issues
  • k-NN bandwidth matters: Too few neighbors → noisy velocity; too many → oversmoothed
  • Sanity check: Root cells (progenitors) should have high unspliced/spliced ratios for marker genes
  • Dynamical model requires distinct kinetic states: Works best for clear differentiation processes
Troubleshooting

| Problem | Solution | |---------|---------| | Missing unspliced layer | Re-run velocyto or use STARsolo with --soloFeatures Gene Velocyto | | Very few velocity genes | Lower min_shared_counts; check sequencing depth | | Random-looking arrows | Try different n_neighbors or velocity model | | Memory error with dynamical | Set n_jobs=1; reduce n_top_genes | | Negative velocity everywhere | Check that spliced/unspliced layers are not swapped |

Additional Resources
  • scVelo documentation: https://scvelo.readthedocs.io/
  • Tutorial notebooks: https://scvelo.readthedocs.io/en/stable/VelocityBasics.html
  • GitHub: https://github.com/theislab/scvelo
  • Paper: Bergen V et al. (2020) Nature Biotechnology. PMID: 32747759
  • velocyto (preprocessing): http://velocyto.org/
  • CellRank (fate prediction, extends scVelo): https://cellrank.readthedocs.io/
  • dynamo (metabolic labeling alternative): https://dynamo-release.readthedocs.io/
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