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Hi y'all,
So I'm trying to detect a CRISPR-induced indel in a specific region of the genome, so I only sequenced that particular region and I was planning on using that specific region as a reference sequence, rather than the whole genome. However, most workflows I've researched involved calling indels against large genomes - which is probably gross overkill for my application.
Does anyone have any thoughts on what would be the best way to detect what percentage of my reads contain an indel within a 500-bp region?
So I'm trying to detect a CRISPR-induced indel in a specific region of the genome, so I only sequenced that particular region and I was planning on using that specific region as a reference sequence, rather than the whole genome. However, most workflows I've researched involved calling indels against large genomes - which is probably gross overkill for my application.
Does anyone have any thoughts on what would be the best way to detect what percentage of my reads contain an indel within a 500-bp region?
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