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  • Solexa mapping - extraction of "not in Ref" reads

    Hi everyone,

    I am searching for a tool/software with which it is possible to map Solexa reads against a reference and which saves the not used reads, too (that's the important part). Is that possible with MAQ?

    Thanks for your help
    Janina

  • #2
    Hi,

    this is possible with bowtie '--un unaligned_reads.fastq'

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    • #3
      CLC Bio's Genomic Workbench does this.

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      • #4
        use maq or bowtie and then pipe their sam output into samtools -f4 - > output.sam

        will keep only the unmapped reads.

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        • #5
          "bowtie --un filename.xxx" will save the unmapped read to a specific file

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          • #6
            maq map -u unmapped_readsFile.txt ...

            gives you the unmapped reads as well
            --
            bioinfosm

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            • #7
              Hi,

              thanks for your help so far! Tried the whole day to understand the SAMtool hint but unfortunately I was not successful. I will describe what I did and maybe someone could help me.

              1: mapping of reads against a reference (Maq)
              2: conversion of Maq output *.map -> *.sam (maq2sam-long)
              3: Sam -> Bam (samtools)
              4: sorted bam file with (samtools)
              5: ./samtools view -f 12 *.sorted bam *.12.bam

              The last step (5) didn't work anymore. It gives no error message but a file with 0 kb (but I know that some reads are not used). I also tried the command with > *.12.bam but nothing happens.
              Has someone an idea? I also tried -f 4 and -f 8 but it is the same... At the end I want to have a fastq file.
              Last edited by Oxygen81; 11-24-2010, 09:21 AM.

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