Additional file 5 of Single nucleotide replacement in the Atlantic salmon genome using CRISPR/Cas9 and asymmetrical oligonucleotide donors

Additional file 5: Figure S4. Illustration of the settings applied for filtering, trimming and variant calling of the MiSeq reads. Fastq files were filtered and trimmed with the following specifications; primer sequences were used to demultiplex reads from different amplicons on the same sequencing...

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Bibliographic Details
Main Authors: Straume, Anne Hege, Kjærner-Semb, Erik, Skaftnesmo, Kai Ove, Güralp, Hilal, Lillico, Simon, Wargelius, Anna, Edvardsen, Rolf Brudvik
Format: Conference Object
Language:unknown
Published: figshare 2021
Subjects:
Online Access:https://dx.doi.org/10.6084/m9.figshare.15041181
https://springernature.figshare.com/articles/presentation/Additional_file_5_of_Single_nucleotide_replacement_in_the_Atlantic_salmon_genome_using_CRISPR_Cas9_and_asymmetrical_oligonucleotide_donors/15041181
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Summary:Additional file 5: Figure S4. Illustration of the settings applied for filtering, trimming and variant calling of the MiSeq reads. Fastq files were filtered and trimmed with the following specifications; primer sequences were used to demultiplex reads from different amplicons on the same sequencing run, minimum read length was set to 100 bp, and forward and reverse reads were assembled to correct sequencing errors (minimum overlap between forward and reverse reads was set to 150 bp for slc45a2 and 200 bp for dnd and allowing at most 20% mismatches between forward and reverse reads in the overlap region). Assembled reads were combined with forward reads that did not pass the assembly thresholds. Variants were then called using positions 20–200 for slc45a2 and positions 60–230 for dnd. All bases with base quality