Entering edit mode
10 months ago
Nodilan
▴
10
Good morning ,
Can I use trimmomatic in order to trim my reads generated using nanopore technology ?
thanks,
Good morning ,
Can I use trimmomatic in order to trim my reads generated using nanopore technology ?
thanks,
Yes, but it probably will not work well, as nanopore read trimming was not Trimmomatics' intended data type.
Have a look at Fastp, chopper or the Porechop_ABI fork of Porechop https://github.com/bonsai-team/Porechop_ABI
Seqtk is another possibility.
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can I still use fastqc and multiqc to check the quality of my nanopore reads ?
While you can, you will want to use a package meant for long reads like PycoQC. It requires the sequencing_summary file from the nanopore run.
You can, but I'd use Fastp and Multiqc instead. Faster and better output of %Q20 and %Q30 reads for ONT (in my opinion). Also PycoQC and or the Nanoplot / Nanopack toolset https://github.com/wdecoster/nanopack might be useful.
This page may help https://help.nanoporetech.com/en/articles/6628901-should-i-qc-my-data-and-what-tools-to-use