Replies: 6 comments
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Looks reasonable. Why? |
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spades.log |
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Everything seems ok to me. Why the results are "puzzling"? |
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As per our experience, such size of data should get more bins with deeper taxonomic annotations , or larger contigs.fasta. This is the first time we try SPAdes based on the literatures and other people's recommendations, so there will be such questions. |
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Hi @SarahIsme, I am curious, how did you chose the kmer parameters? Best wishes, |
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Dear @franciscozorrilla , Sorry for the late reply. Yes, after filtration by checkM, the number of bins will be lower. Best regards, Mort |
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Dear developers,
I used two paired-end reads trimmed by Trimmomatic. The forward read was 18 GB and the reverse read was 17.8 GB. The command was:
/miniconda3/bin/spades.py --meta -1 forward.fq.gz -2 reverse.fq.gz -t 16 -m 40 -k 55,77,99 -o outfile
.However the contigs.fasta was 132MB and scaffolds.fasta was also 132MB. Then the contigs.fasta was used for binning by concoct, maxbin2 and metabat2, there were only 48, 28 and 36 bins, respectively.
Is there some parameters wrong in my command line for SPAdes?
Thanks in advance!
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