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  • sequenced transcriptome- how do I identify my transcripts

    Aligned to mm10 using bowtie2, and converted to a sorted bam using samtools. How do I analyze my reads and what transcripts they correspond to

  • #2
    I'd drop the bowtie2 and instead use Tophat2 (which granted, will use bowtie2 internally but will also do better analysis).

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    • #3
      or Mira or Newbler

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      • #4
        Originally posted by westerman View Post
        I'd drop the bowtie2 and instead use Tophat2 (which granted, will use bowtie2 internally but will also do better analysis).
        I had a question about that. Does bowtie2 throw reads out if they overlap at a splice junction since you're referencing to a genome ?

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        • #5
          Originally posted by KnowNothing2 View Post
          I had a question about that. Does bowtie2 throw reads out if they overlap at a splice junction since you're referencing to a genome ?
          Depends on what command line parameters you use. Within some limitations ' --local' will map the read to either side of the splice but you will have to force the program to show more than the 'best' alignment via '-k' or '-a'.

          I point out that Tophat2 does not use '--local' but rather '--end-to-end'. It can do this because it actually splits up reads into smaller segments that should map end-to-end and not need the soft-clipping that 'local' generates.

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