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  • how can I get abundance from both Iso-seq output and illumina data?

    Hi,
    We've got the done the RNA-seq of a species (genome is about 3GB), but NO reference genome is available, using pacbio and Illumina. After the RS_IsoSeq and cd-hit analysis, we have redundant full-length transcripts. Now we want to get the quantification using short reads with Iso-*Seq output used as reference. Since we don't have reference genome, several method can be considered:
    1. RSEM( bowtie+RSEM)
    2. RSEM (bowtie+eXpress)
    3. blat +counting reads mapped to full-length transcript

    But now I am confused which method is best for the quantification? Or is there any other method to quantify for no-reference species?

    Thanks a lot for any apply!
    happy

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