I have a set of 454 amplicon data that comprises six multiplexed (barcoded) samples.
I've already processed and analysed this data through Qiime, but I'm currently trying to get the raw reads uploaded in the NCBI SRA.
I can upload the data as a single .sff file, but it would make more sense to demultiplex it first and upload separate fatsq files for each sample.
I tried converting the sff. to fastq using mothur, then running split_libraries_fastq.py in Qiime, but because this is 454 data, not Illumina, I don't have separate barcode read fastq files, so the script won't work.
Can anyone help me with this?
I've already processed and analysed this data through Qiime, but I'm currently trying to get the raw reads uploaded in the NCBI SRA.
I can upload the data as a single .sff file, but it would make more sense to demultiplex it first and upload separate fatsq files for each sample.
I tried converting the sff. to fastq using mothur, then running split_libraries_fastq.py in Qiime, but because this is 454 data, not Illumina, I don't have separate barcode read fastq files, so the script won't work.
Can anyone help me with this?
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