Hello, While I'm aware its not the best tool for detecting relatively small CNVs, I'm trying to use CNVKit to detect a single exon deletions. I have a very small panel of genes (~10) with very high coverage (>1000). However when I run

cnvkit.py coverage sample123.bam one_row.bed -o sample123.cnn

where one_row.bed has a single regions spanning few bases (I tried 200 bases and 5 bases). I'm looking at the bam file and each base in this region has >1000 depth, but still, the depth in the cnn output file is very low (~10).

What am I missing? Shouldn't the depth hold the average depth of all the bases in the region?

Thank you for the help.

Are most of the reads marked as duplicates? Those wouldn't be counted. You could also try the -c option with the coverage command to get roughly the same answer calculated through a different method.

In CNVkit 0.8.3 you can use the bundled script coverage_bin_size.py to estimate ideal bin sizes based on the coverage depth in a given sample. This most recent version also includes some internal improvements to handle targeted amplicon sequencing better.

For single-exon detection: As a wild guess, I'd try an average target bin size of 40 or 50, and run segmentation with the HaarSeg method (segment -m haar). Also, be sure to run the fix and reference commands with the option --no-edge, and perhaps also --no-gc --no-rmask if your target footprint is very small.