Dear all,
I have metagenomic data which was produced from Illumina HiSeq 100 PE sequencing. After de novo assembly using velvet with a range of kmers, I came up with one kmer. When I looked at the percent of reads used for assembly, 70% of reads were actually used. I got curious what people are doing with the rest of 30% of unused reads and looked into threads related to this but haven't got a clear idea. Could anyone give me some advice or direct me any publication? Thanks!
I have metagenomic data which was produced from Illumina HiSeq 100 PE sequencing. After de novo assembly using velvet with a range of kmers, I came up with one kmer. When I looked at the percent of reads used for assembly, 70% of reads were actually used. I got curious what people are doing with the rest of 30% of unused reads and looked into threads related to this but haven't got a clear idea. Could anyone give me some advice or direct me any publication? Thanks!
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