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  • GeneJockey
    Junior Member
    • May 2012
    • 4

    Bowtie signal 9 (KILL) error

    I'm aligning a bunch of Illumina runs using Bowtie2 and I'm getting a frustrating error with only a few of the fastq files.

    I run them with the following command:

    bowtie2 -p 10 -x mm10_genome -1 SRR594396_1.fastq -2 SRR594396_2.fastq --local --very-sensitive-local --no-mixed --no-discordant | samtools view -uS - | samtools sort -m 10000000000 - SRR594393_genome

    Here are the outputs I get for a few fastq file pairs:

    SRR594399_genome
    [samopen] SAM header is present: 22 sequences.
    Parse error at line 111594048: missing colon in auxiliary data
    [bam_sort_core] merging from 2 files...

    SRR594400_genome
    [samopen] SAM header is present: 22 sequences.
    bowtie2-align died with signal 9 (KILL)
    [sam_read1] reference 'SRR59' is recognized as '*'.
    [main_samview] truncated file.
    [bam_sort_core] merging from 2 files...

    SRR594401_genome
    [samopen] SAM header is present: 22 sequences.
    Parse error at line 111266936: sequence and quality are inconsistent
    [bam_sort_core] merging from 2 files...

    SRR594396_genome
    [samopen] SAM header is present: 22 sequences.
    bowtie2-align died with signal 9 (KILL)
    Parse error at line 111938538: missing colon in auxiliary data
    [bam_sort_core] merging from 2 files...

    SRR594415_genome
    [samopen] SAM header is present: 22 sequences.
    bowtie2-align died with signal 9 (KILL)
    Parse error at line 112131890: missing colon in auxiliary data
    [bam_sort_core] merging from 2 files...

    SRR594417_genome
    [samopen] SAM header is present: 22 sequences.
    bowtie2-align died with signal 9 (KILL)
    Parse error at line 112044487: sequence and quality are inconsistent
    [bam_sort_core] merging from 2 files...

    I can't find anything about this KILL error and googling the parse errors isn't helping much. I think the parsing has something to do with bowtie failing and then the sam->bam operation subsequently failing on the last line.

    Can anyone help with this KILL business?
  • anthony_h
    Junior Member
    • Nov 2013
    • 2

    #2
    Also getting KILL

    I am also getting this when I turn on the -a option.

    Without -a my file of ~7M reads gets mapped against human genome hg19 successfully. With -a it bombs out even if I truncate to 200k reads. Maybe the process is using too much memory and the OS is killing it?

    Comment

    • davidblaney
      Member
      • Nov 2011
      • 18

      #3
      I was thinking a memory issue when I first read this. Have a look at the requirement on there website. Failing that drop them an email.

      Comment

      • ctseto
        Member
        • Oct 2013
        • 44

        #4
        What happens when you use --local --very-sensitive-local at the same time? I assume it picks one and keeps on going?

        Comment

        • Richard Finney
          Senior Member
          • Feb 2009
          • 701

          #5
          How much memory does you system have?

          System may kill processes if there is severe resource starvation; i.e. no memory available.

          Comment

          • anthony_h
            Junior Member
            • Nov 2013
            • 2

            #6
            Yes, it was running out of memory.

            Switched to using -k instead of -a and it completed.

            Comment

            • jylee
              Junior Member
              • Jun 2019
              • 3

              #7
              Hi all,
              I am encountering same issue SIGNAL 9 (KILL). I wonder how you solved this issue.

              Anthony h,
              Could you describe more detail how you set -k <int> options?

              Comment

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