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  • sudarynja3
    Junior Member
    • Jan 2011
    • 2

    TopHat "junction" error

    Hi I have some wey strange error.
    I run ~200 samples with tophat2 and 7 do not run with following error:
    ___________________________________________________________________
    tophat2 -p 8 --read-mismatches 4 -o thaln_HV ~/HV_consensus.fa unmapped.fq

    [2012-10-09 12:01:43] Beginning TopHat run (v2.0.0)
    -----------------------------------------------
    [2012-10-09 12:01:43] Checking for Bowtie
    Bowtie version: 2.0.0.6
    [2012-10-09 12:01:43] Checking for Samtools
    Samtools version: 0.1.18.0
    [2012-10-09 12:01:43] Checking for Bowtie index files
    [2012-10-09 12:01:43] Checking for reference FASTA file
    [2012-10-09 12:01:43] Generating SAM header for HV_consensus.fa
    format: fastq
    quality scale: phred33 (default)
    [2012-10-09 12:01:43] Preparing reads
    left reads: min. length=18, count=515457
    Warning: short reads (<20bp) will make TopHat quite slow and take large amount of memory because they are likely to be mapped to too many places
    [2012-10-09 12:01:58] Mapping left_kept_reads against HV_consensus.fa with Bowtie2
    [2012-10-09 12:02:40] Mapping left_kept_reads_seg1 against HV_consensus.fa with Bowtie2 (1/3)
    [2012-10-09 12:02:47] Mapping left_kept_reads_seg2 against HV_consensus.fa with Bowtie2 (2/3)
    [2012-10-09 12:02:54] Mapping left_kept_reads_seg3 against HV_consensus.fa with Bowtie2 (3/3)
    [2012-10-09 12:02:59] Searching for junctions via segment mapping
    Warning: junction database is empty!
    [2012-10-09 12:03:07] Retrieving sequences for splices
    [2012-10-09 12:03:07] Indexing splices
    Warning: Empty fasta file: 'thaln_HV/tmp/segment_juncs.fa'
    Warning: All fasta inputs were empty
    Error: Encountered internal Bowtie 2 exception (#1)
    Command: /bin/bowtie2-2.0.0-beta6/bowtie2-build thaln_HV/tmp/segment_juncs.fa thaln_HV/tmp/segment_juncs
    [FAILED]
    Error: Splice sequence indexing failed with err =1
    _____________________________________________

    strange thing is if i use --no-novel-junc option it runs ... even though i actually do not specify GTF file .....
    my reference is mixed fasta file for metagenomic study and it works fine for other samples. So i assume something is wrong with my *fq file, but they look fine, and reads phred quality is >= 30

    anyone can help with the mystery?

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