Low number of reads aligned #449
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Hi, Amplicon without edition: sgRNA: APOE44-STINGII-CR-clone-1-DB-FR-NIM_S80_L001_R1_001.fastq.gz Thanks for your response, |
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Replies: 3 comments 2 replies
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Hi Frances, Thanks for using CRISPResso! If you suspect you have a large deletion, I bet that reads are not meeting the default 60% homology cutoff. I would recommend setting the Let us know if this works for you! Thanks, |
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Thanks a lot Colelyman for your quick reply. I will try that! Frances |
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Hi Colelyman, I don't find where I can change the cut off to 0. In"options" I find 50, 60, 70, 80, 90 and 100%: Thanks Frances |
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Sorry about that, I didn't realize you are using the web version. You can only set the score that low through the command line version. I have run the following command on your data and the results are attached (note that 100% of the reads are now aligned). I didn't look too closely, but I would make sure that your amplicon sequence is correct (all of the primers removed, etc.). |
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Thanks Cole for your reply. I will ask for help to use the command line version in the bioinformatics core. The primers were not removed. So I would take this into account. |
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Hi Frances,
Thanks for using CRISPResso! If you suspect you have a large deletion, I bet that reads are not meeting the default 60% homology cutoff. I would recommend setting the
--default_min_aln_scoreparameter to 0, then every read that passes preprocessing will be aligned.Let us know if this works for you!
Thanks,
Cole