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  • #1

    how to filter a bam file

    Dear All,
    I am facing a problem with huge rRNA and globin RNA contamination in my SOLiD data (colour space format csfasta)
    I would like now to get rid of this reads in my csfasta files or in my bam file ( I used tophat to align).
    I s there a way to delete those reads from either the files?
    Any suggestions will be appreciated,
    Paolo
    Tags: None
  • #2
    I like to do it with BEDTools; I use "intersectBed -v" to remove the reads mapping to rRNA regions (given in a GFF file).

    First get the GFF with rRNA regions:
    Code:
    grep -P "\trRNA\t" annotation.gff > rRNAs.gff
    You might need to adapt the matching pattern here, works fine with e.g. Arabidopsis TAIR10 GFF3.

    Then get all reads not intersecting with these regions:
    Code:
    intersectBed -v -abam tophat_aligned_reads.bam -b rRNAs.gff > tophat_aligned_reads_no_rRNAs.bam
    Last edited by arvid; 01-19-2012, 02:24 AM. Reason: esthetic

    Comment

    • #3
      thanks for your help I get rid of my junk sequences!

      Comment

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