Demultiplexing MinION reads
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3.8 years ago
jeccy.J ▴ 60

Hi Community,

I have run Guppy on naopore reads for the basecalling and generated a final merged fastq file. Next, for demultiplexing I have seen a couple of option available, such as Porechop, Last and qcat. Can anyone suggest me from their earlier experience which tool I should use for demultiplexing of the basecalled fastq reads? As an input data i have the a .fastq file and one fasta file with all the barcode.

JC
demutiplex • 6.4k views
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3.8 years ago
shelkmike ★ 1.4k

I use Porechop and I have no problems with it.
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Could you please let me know the running command. I checked the manual it looks like : porechop -i input_reads.fastq.gz -b output_dir here, how i should provide my input barcode fasta file?

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https://github.com/rrwick/Porechop#barcode-demultiplexing

Scroll down at the link above. Looks like you need to edit adapters.py script and add them if you use custom barcodes.

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Do you use Guppy for basecalling or any other tool?

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Sorry, I didn't notice your first comment. You should manually edit the adapters.py file to add barcodes. I use guppy for basecalling and then porechop for demultiplexing or trimming when non-standard adapters are used.

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2.9 years ago

I think the generally accepted and most up to date tool to use is

guppy_barcoder

from ONT

Usage is quite easy (it runs on fastq files output by guppy, not on FAST5 files).
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