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  • count reads number in collapsed file

    Hi all,

    I used bowtie to align a collapsed fasta file to the bovine genome and get a fasta file (mapped.fa) including all the mapped reads. But this mapped.fa is also a collapsed file. So how could I get the total reads number in mapped.fa, instead of the unique reads number?

    Thanks.

    Ran

  • #2
    What do you mean by "collapsed"? Could you copy and paste the exact commands that were run?

    Comment


    • #3
      Hi Heisman, thanks for your reply. The collapsed file included the unique reads:

      >1-30176523
      TCAGTGCACTACAGAACTTTGT
      >2-17234938
      TTCAAGTAATCCAGGATAGGCT
      >5-10273189
      TACCCTGTAGAACCGAATTTGT
      >6-10202799
      TGAGATGAAGCACTGTAGCT
      >7-7833696
      TGAGATGAAGCACTGTAGCTCT
      >8-7677783
      TGTAAACATCCTCGACTGGA
      >9-7403197
      TGTAAACATCCTCGACTGGAAGCT
      >10-5760993
      TGGGGGGCCCAAGTCCTTCTGATCGAGGCC

      So here I can get the number of total unique reads. But each unique read represents thousands of reads. How could I get the total number of the redundant reads in this file?

      Thanks!

      Comment

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