Good morning everyone,

I hope someone can help me with this issue. In my lab, we performed a targeted sequencing with Illumina MiSeq. We sequenced one single gene (whole gene, both introns and exons) in 96 samples, belonging to two different experimental groups. After the alignment and the duplicates removal, I decided to visualize my bam files using the Golden Helix Genome Browser. I noticed a reduction of the coverage for a 200bp region in the only coding exon of my sequenced gene. This reduction occurs in all my samples but it is more evident in one group than the other (statistically determined using read depth values).

How should I interpret these data?

It is a deletion!

(seriously, it is not a reduction of coverage, but a massive drop of 50% at exactly two bases, instead of gradual reduction)

I recommend to load it to IGV and inspect soft-clipped parts of reads and paired-end distances

There are several reasons why this could be happening. One of the easiest and fastest ones to check is that maybe that coding exon has an homolog region in the genome, therefore some reads may be mapping with equal probability on both sites (this assigns those reads a mapping quality of "0"). Check if reads with mapping quality = 0 are being filtered (maybe only reads with mapping quality > 1 are being displayed by default) and, if so, just remove that threshold and check if the coverage on that region changes. If it does you'll know the reason why, and if doesn't you may continue thinking about other alternatives.