single-cell-rna-qc
Performs quality control on single-cell RNA-seq data (.h5ad or .h5 files) using scverse best practices with MAD-based filtering and comprehensive visualizations.
Best use case
single-cell-rna-qc is best used when you need a repeatable AI agent workflow instead of a one-off prompt.
Performs quality control on single-cell RNA-seq data (.h5ad or .h5 files) using scverse best practices with MAD-based filtering and comprehensive visualizations.
Teams using single-cell-rna-qc should expect a more consistent output, faster repeated execution, less prompt rewriting.
When to use this skill
- You want a reusable workflow that can be run more than once with consistent structure.
When not to use this skill
- You only need a quick one-off answer and do not need a reusable workflow.
- You cannot install or maintain the underlying files, dependencies, or repository context.
Installation
Claude Code / Cursor / Codex
Manual Installation
- Download SKILL.md from GitHub
- Place it in
.claude/skills/single-cell-rna-qc/SKILL.mdinside your project - Restart your AI agent — it will auto-discover the skill
How single-cell-rna-qc Compares
| Feature / Agent | single-cell-rna-qc | Standard Approach |
|---|---|---|
| Platform Support | Not specified | Limited / Varies |
| Context Awareness | High | Baseline |
| Installation Complexity | Unknown | N/A |
Frequently Asked Questions
What does this skill do?
Performs quality control on single-cell RNA-seq data (.h5ad or .h5 files) using scverse best practices with MAD-based filtering and comprehensive visualizations.
Where can I find the source code?
You can find the source code on GitHub using the link provided at the top of the page.
SKILL.md Source
# Single-Cell RNA-seq Quality Control
Automated QC workflow for single-cell RNA-seq data following scverse best practices.
## When to Use This Skill
Use when users:
- Request quality control or QC on single-cell RNA-seq data
- Want to filter low-quality cells or assess data quality
- Need QC visualizations or metrics
- Ask to follow scverse/scanpy best practices
- Request MAD-based filtering or outlier detection
**Supported input formats:**
- `.h5ad` files (AnnData format from scanpy/Python workflows)
- `.h5` files (10X Genomics Cell Ranger output)
**Default recommendation**: Use Approach 1 (complete pipeline) unless the user has specific custom requirements or explicitly requests non-standard filtering logic.
## Approach 1: Complete QC Pipeline (Recommended for Standard Workflows)
For standard QC following scverse best practices, use the convenience script `scripts/qc_analysis.py`:
```bash
python3 scripts/qc_analysis.py input.h5ad
# or for 10X Genomics .h5 files:
python3 scripts/qc_analysis.py raw_feature_bc_matrix.h5
```
The script automatically detects the file format and loads it appropriately.
**When to use this approach:**
- Standard QC workflow with adjustable thresholds (all cells filtered the same way)
- Batch processing multiple datasets
- Quick exploratory analysis
- User wants the "just works" solution
**Requirements:** anndata, scanpy, scipy, matplotlib, seaborn, numpy
**Parameters:**
Customize filtering thresholds and gene patterns using command-line parameters:
- `--output-dir` - Output directory
- `--mad-counts`, `--mad-genes`, `--mad-mt` - MAD thresholds for counts/genes/MT%
- `--mt-threshold` - Hard mitochondrial % cutoff
- `--min-cells` - Gene filtering threshold
- `--mt-pattern`, `--ribo-pattern`, `--hb-pattern` - Gene name patterns for different species
Use `--help` to see current default values.
**Outputs:**
All files are saved to `<input_basename>_qc_results/` directory by default (or to the directory specified by `--output-dir`):
- `qc_metrics_before_filtering.png` - Pre-filtering visualizations
- `qc_filtering_thresholds.png` - MAD-based threshold overlays
- `qc_metrics_after_filtering.png` - Post-filtering quality metrics
- `<input_basename>_filtered.h5ad` - Clean, filtered dataset ready for downstream analysis
- `<input_basename>_with_qc.h5ad` - Original data with QC annotations preserved
If copying outputs for user access, copy individual files (not the entire directory) so users can preview them directly.
### Workflow Steps
The script performs the following steps:
1. **Calculate QC metrics** - Count depth, gene detection, mitochondrial/ribosomal/hemoglobin content
2. **Apply MAD-based filtering** - Permissive outlier detection using MAD thresholds for counts/genes/MT%
3. **Filter genes** - Remove genes detected in few cells
4. **Generate visualizations** - Comprehensive before/after plots with threshold overlays
## Approach 2: Modular Building Blocks (For Custom Workflows)
For custom analysis workflows or non-standard requirements, use the modular utility functions from `scripts/qc_core.py` and `scripts/qc_plotting.py`:
```python
# Run from scripts/ directory, or add scripts/ to sys.path if needed
import anndata as ad
from qc_core import calculate_qc_metrics, detect_outliers_mad, filter_cells
from qc_plotting import plot_qc_distributions # Only if visualization needed
adata = ad.read_h5ad('input.h5ad')
calculate_qc_metrics(adata, inplace=True)
# ... custom analysis logic here
```
**When to use this approach:**
- Different workflow needed (skip steps, change order, apply different thresholds to subsets)
- Conditional logic (e.g., filter neurons differently than other cells)
- Partial execution (only metrics/visualization, no filtering)
- Integration with other analysis steps in a larger pipeline
- Custom filtering criteria beyond what command-line params support
**Available utility functions:**
From `qc_core.py` (core QC operations):
- `calculate_qc_metrics(adata, mt_pattern, ribo_pattern, hb_pattern, inplace=True)` - Calculate QC metrics and annotate adata
- `detect_outliers_mad(adata, metric, n_mads, verbose=True)` - MAD-based outlier detection, returns boolean mask
- `apply_hard_threshold(adata, metric, threshold, operator='>', verbose=True)` - Apply hard cutoffs, returns boolean mask
- `filter_cells(adata, mask, inplace=False)` - Apply boolean mask to filter cells
- `filter_genes(adata, min_cells=20, min_counts=None, inplace=True)` - Filter genes by detection
- `print_qc_summary(adata, label='')` - Print summary statistics
From `qc_plotting.py` (visualization):
- `plot_qc_distributions(adata, output_path, title)` - Generate comprehensive QC plots
- `plot_filtering_thresholds(adata, outlier_masks, thresholds, output_path)` - Visualize filtering thresholds
- `plot_qc_after_filtering(adata, output_path)` - Generate post-filtering plots
**Example custom workflows:**
**Example 1: Only calculate metrics and visualize, don't filter yet**
```python
adata = ad.read_h5ad('input.h5ad')
calculate_qc_metrics(adata, inplace=True)
plot_qc_distributions(adata, 'qc_before.png', title='Initial QC')
print_qc_summary(adata, label='Before filtering')
```
**Example 2: Apply only MT% filtering, keep other metrics permissive**
```python
adata = ad.read_h5ad('input.h5ad')
calculate_qc_metrics(adata, inplace=True)
# Only filter high MT% cells
high_mt = apply_hard_threshold(adata, 'pct_counts_mt', 10, operator='>')
adata_filtered = filter_cells(adata, ~high_mt)
adata_filtered.write('filtered.h5ad')
```
**Example 3: Different thresholds for different subsets**
```python
adata = ad.read_h5ad('input.h5ad')
calculate_qc_metrics(adata, inplace=True)
# Apply type-specific QC (assumes cell_type metadata exists)
neurons = adata.obs['cell_type'] == 'neuron'
other_cells = ~neurons
# Neurons tolerate higher MT%, other cells use stricter threshold
neuron_qc = apply_hard_threshold(adata[neurons], 'pct_counts_mt', 15, operator='>')
other_qc = apply_hard_threshold(adata[other_cells], 'pct_counts_mt', 8, operator='>')
```
## Best Practices
1. **Be permissive with filtering** - Default thresholds intentionally retain most cells to avoid losing rare populations
2. **Inspect visualizations** - Always review before/after plots to ensure filtering makes biological sense
3. **Consider dataset-specific factors** - Some tissues naturally have higher mitochondrial content (e.g., neurons, cardiomyocytes)
4. **Check gene annotations** - Mitochondrial gene prefixes vary by species (mt- for mouse, MT- for human)
5. **Iterate if needed** - QC parameters may need adjustment based on the specific experiment or tissue type
## Reference Materials
For detailed QC methodology, parameter rationale, and troubleshooting guidance, see `references/scverse_qc_guidelines.md`. This reference provides:
- Detailed explanations of each QC metric and why it matters
- Rationale for MAD-based thresholds and why they're better than fixed cutoffs
- Guidelines for interpreting QC visualizations (histograms, violin plots, scatter plots)
- Species-specific considerations for gene annotations
- When and how to adjust filtering parameters
- Advanced QC considerations (ambient RNA correction, doublet detection)
Load this reference when users need deeper understanding of the methodology or when troubleshooting QC issues.
## Next Steps After QC
Typical downstream analysis steps:
- Ambient RNA correction (SoupX, CellBender)
- Doublet detection (scDblFinder)
- Normalization (log-normalize, scran)
- Feature selection and dimensionality reduction
- Clustering and cell type annotationRelated Skills
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