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  • picrinite
    Junior Member
    • Feb 2015
    • 2

    Preparing reads in TopHat

    Dear Friends,

    When I run tophat to align RNA-Seq reads, the log file shows that some reads are discarded as below. Does anyone know why they are discarded? low quality reads? How can I setup the threshold for reads discarding?

    Thank you very much.


    [2015-01-25 22:24:21] Beginning TopHat run (v2.0.8b)
    -----------------------------------------------
    [2015-01-25 22:24:21] Checking for Bowtie
    Bowtie version: 2.1.0.0
    [2015-01-25 22:24:21] Checking for Samtools
    Samtools version: 0.1.19.0
    [2015-01-25 22:24:21] Checking for Bowtie index files
    [2015-01-25 22:24:21] Checking for reference FASTA file
    [2015-01-25 22:24:21] Generating SAM header for musculus
    format: fastq
    quality scale: phred33 (default)
    [2015-01-25 22:24:44] Reading known junctions from GTF file
    [2015-01-25 22:24:48] Preparing reads
    left reads: min. length=101, max. length=101, 6682858 kept reads (653 discarded)
    right reads: min. length=101, max. length=101, 6641398 kept reads (42113 discarded)
  • Brian Bushnell
    Super Moderator
    • Jan 2014
    • 2709

    #2
    Considering it's mainly read 2 being discarded, looks like low-quality reads. You might get better results by quality-trimming the data first, as Tophat is not very tolerant of errors; that may also reduce the number of reads discarded. Removing the last base of 101bp reads is also a good idea, IMO.

    Comment

    • picrinite
      Junior Member
      • Feb 2015
      • 2

      #3
      Thank you.
      Yes, if reads are filtered first, only 20 reads are discarded by tophat.
      I have tried reading tophat manual but no information about tophat's default filtering parameters is found.

      Comment

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