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  • Illumina reads pretreatmentS before de-novo transcriptome assembly

    Hello everybody,

    Lately with datasets of >1bio 100 bp SE reads, I have been using these steps to do de-novo assembly of a complex eukaryotic genome (without a good quality genome, diploid with a high degree of single nucleotide polymorphism, which further complicate the assembly):

    1. Adapter removal (I usually use adaperRemoval http://www.ncbi.nlm.nih.gov/pubmed/22748135 )
    2. Error correction (http://sb.cs.cmu.edu/seecer/)
    3. Digital normalization (http://arxiv.org/abs/1203.4802) -
    I then usually assemble using velvet/oases

    Individually I made some test and found all of these steps efficients and useful, but I guess I am not involved enough in the details of algorithms used to come up with a optimal order in which to use them.

    In your opinion, is the order I*propose a good one to produce a decent transcriptome ?

    In advance, many thanks for your insights !

    Yvan

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