I've sequenced targeted DNA panel. I'm aligning it using bwa mem once to the whole genome and twice to the targeted sequences. When aligning it to the reference genome I'm getting ~30% of the reads mapped to the targeted regions. However, when aligning it to the panel sequences 70% of the read are aligned successfully.

Any idea how can it happen? even if there is favored alignment in the whole genome these reads should be assigned as supplementary alignment? Isn't it?

Hello,

there are only secondary alignments (not supplementary) if the probability of these alignments are similar. So in your whole genome alignment lots of your reads maps significantly better to other regions, than the one you guess.

That's a very good example why you should always align to the whole genome, even if you use panels.

fin swimmer

The sequences of the target regions of your panel is not unique. So always align to the whole genome, or you have to confirm that the primers of the panel are unique.