Entering edit mode
4.6 years ago
1769mkc
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1.2k
I have 16s rna meta-genomic sequence data. So far I have done is basecalling using guppy which resulted in fastq files. A total of 96 samples were sequenced.
- I have 96 barcoding folder and inside each folder there are 1962 fastq files.
So do I merge all the fastq reads and make them one file or each file are analysed individually
Few of the pipelines I have read so far for nanopore reads,one of them is this. I would like to assign taxonomic labels to these samples which can be done using kraken or centrifuge. Is it possible to use either of these tools with the above pipeline?
NCBI now has 16S/18S/ITS/LSU/SSU pre-formatted blast databases. You could try those out.
surely i will use that but right now Im in pre processing step of the data I will find out about the primers and update
Are these amplicons done using degenerate primers?
I will have to find out what primer we have used
No these are not degenerate primers . How to go about it since there are about 1962 fastq files under each barcoding how to go about it. Should I merge all the fastq files and proceed?
Since we don't know how these were generated and/or what region you are looking at from 16S you could do the following.
Actually we started using that epi2me and WIMP when we had less sequence since that happens all in the server side it takes a lot of time then only we started looking how to do locally.
"what region you are looking at from 16S " This I will update