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  • RNA-SEQ with SOLID reads

    Hi
    I have Solid reads of length 75 x 35
    I want to use Tophat and cufflinks to analyze these reads. But the problem is I dont have the fastq files. I have already mapped reads in BAM format.
    should I re-run tophat on these mapped reads? and how?
    and which library type I should use? and how ?

    /dnyansagar

  • #2
    Hello, you can try this tool:

    http://www.hudsonalpha.org/gsl/software/bam2fastq.php

    Be careful though to read carefully the assumtions, and then, when you will run tophat, take into account what is said to the instructions about the Phred scale.

    Comment


    • #3
      Hello, you can try this tool:

      http://www.hudsonalpha.org/gsl/software/bam2fastq.php

      Be careful though to read carefully the assumtions, and then, when you will run tophat, take into account what is said to the instructions about the Phred scale.

      Comment


      • #4
        Hello
        I have another question. I am new to RNA-seq and therefore the question is sort of basic.
        I have Drosophila Solid reads. The experiment have 3 controls (2 wild type and 1 gene specific)and an experiment each having 6 files. I am using Tophat-Cufflinks for the study. My question is, should I use all 18 control files to compare against ?

        Comment

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