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  • Is this assembly reasonable?

    I have completed some de novo assemblies of MiSeq generated 250PE reads with Minia and SSPACE. I've posted a description of the outcomes and some quality checks at the following site:

    http://www.dartergenomics.org/tallapoosa-darter-genome

    For those of you with experience in assemblies, could you please look this over and let me know if the scaffold distributions I ended up with are reasonable given the MiSeq data?

    Thanks.

  • #2
    As an author of Minia, I would say that it looks good, but I would be a bit biased Thanks for using the software.

    The k=73 min_abundance=2 assembly appears to be better than the k=63 min_abundance=3, consistently over all metrics. Thus you could focus on the k=73 one.

    I have not tested them, but two tools can help you further evaluate accuracy metrics of an assembly without a reference:

    Wellcome Sanger Institute tools directory


    Also you mentioned that there are ~53M paired reads, yielding 13x coverage. Does each of the 53M paired reads consist of two mates of length 250bp? if so the coverage should be multiplied by two.

    Comment


    • #3
      Thanks for the references.

      And to be clear, there are 53 million individual reads.

      Comment

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