Porechop demulitplexing of nanopore sequencing data and barcode bins for each sample

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6 months ago

muhammad.akram ▴ 10

Dear, I am new to nanopore community and have some questions. I might sound silly! We preapred nanopore librariy using 1-24 SQK-16S024 kit for 24 samples. After sequencing, i got fast5 and fastq files. Fastq files were subjected to Porechop for demultiplexing and adapter trimming. As an output, porechop created only 2 barcode bins, BC01 and BC02. BC01 is a very big file with more than 1 million reads. The question is how many barcode bins were expected after porechop process as we created 24 sample library? I was expecting 24 barcode bins as i used 24 samples for the library preparation. COuld you please share your experience, it might be helpful. Thanks!

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ADD COMMENT • link updated 6 months ago by samuel.a.odonnell ▴ 520 • written 6 months ago by muhammad.akram ▴ 10

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While the kit is for 24 samples, how many barcodes did you actually use?

ADD REPLY • link 6 months ago by andres.firrincieli 3.6k

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OP says:

I was expecting 24 barcode bins as i used 24 samples for the library preparation.

ADD REPLY • link 6 months ago by GenoMax 141k

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Considering you barcoded 24 samples, you should expect 24 barcode bins as you stated.

I am not sure porechop has the barcodes for the kit you have used. This might be your issue. You should try using the demultiplexing in guppy instead anyway

ADD REPLY • link 6 months ago by samuel.a.odonnell ▴ 520

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