Route: chip
ChIP-seq analysis.
Segments:
- Align to the reference genome (Bowtie2).
- Remove duplicate reads (Sambamba).
- Generate genome browser tracks.
For peak calling, follow with chip-pairs-peaks.
Usage
Set up a new analysis (common across all routes). If running for the first time, check the detailed usage instructions for an explanation of every step.
cd <project dir>
git clone --depth 1 https://github.com/igordot/sns
sns/generate-settings <genome>
sns/gather-fastqs <fastq dir>
Run chip
route.
sns/run chip
Check for potential problems.
grep "ERROR:" logs-sbatch/*
Output
Primary results:
BAM-DD
: Deduplicated BAM files. Can be used for additional analysis.BIGWIG
: BigWig files normalized to the total number of reads. Can be used for visual inspection of peaks.
Run metrics:
summary-combined.chip.csv
: Summary table that includes the number of reads, alignment rate, and fraction of PCR duplicates.