Hi!

I'm having a issue demultiplexing a fastq file containing multiple samples from a nextseq run. we had dual index and dual barcode for each sample. the demultiplexing on the index (I5 and i7) worked properly but I still need to demultplex the barcode_5 and barcode_7. it goes like this:

The "NNNNNN" sequence are the barcode I have to demultiplex to get individual samples.

I have a list of barcode per samples. Here is some examples:

Sample_ID Barcode_5 Sequence 5'-3' Barcode_7 Sequence 5'-3'

A_1 501 TCCGATAT 701 GCTCATTAT

A_2 502 CGGAGATA 701 GCTCATTAT

I saw that nextseq use barcode reverse complement so I tried to dempultiplex using the following:

A_1 TCCGATAT-ATAATGAGC

A_2 CGGAGATA-ATAATGAGC

but all the reads went to the unmatched fastq. I then tried to use the exact sequence I was given.

A_1 TCCGATAT-GCTCATTAT

A_2 CGGAGATA-GCTCATTAT

but it didn't work either...

I can't figure out what I did wrong... Is there another tool that can demultiplex this kind of dual barcoded reads?

By two barcodes at once, you mean the two inner barcodes ("NNNNN", barcode_5 and barcode_7), right? Cutadapt actually supports demultiplexing in addition to trimming, and I think it might be able to do this. In particular see the bit about combinatorial dual indexes.

So for example if you have a read pair like this (just using FASTA for a dumb example)

r1.fasta:

>seq1
GGGGGGGACTGACTG
>seq2
GGGGGGGAGAGACGC
>seq3
TTTTTTTCTCTGAGA
>seq4
TTTTTTTCAAACTTA

r2.fasta:

>seq1
AAAAAAACAGTCAGT
>seq2
GGGGGGGGCGTCTCT
>seq3
AAAAAAATCTCAGAG
>seq4
GGGGGGGTAAGTTTG

...and barcodes like this...

barcodes_fwd.fasta:

>fwd1
GGGGGGG
>fwd2
TTTTTTT

barcodes_rev.fasta:

>rev1
AAAAAAA
>rev2
GGGGGGG

You can do this:

$ cutadapt -e 0.15 --no-indels -g ^file:barcodes_fwd.fasta -G ^file:barcodes_rev.fasta \
    -o {name1}-{name2}.1.fasta -p {name1}-{name2}.2.fasta \
    r1.fasta r2.fasta

... and each of those four pairs of sequences will end up in a separate pair of files named like fwd1-rev1.1.fasta etc.