Tophat-Fusion Error 'Long_Spanning_Reads'
1
0
Entering edit mode
11.8 years ago
samsara ▴ 630

I have run Tophat fusion with paired-end RNA-Seq data, but my run was unsuccessful. The error says running 'long_spanning_reads'. I found a post in SEQanswers, but it did not help much.

Following is the executed command.

tophat -o $DIRECTORY$SAMPLENAME \
-p 16 \
--fusion-search \
--keep-fasta-order \
--bowtie1 \
--no-coverage-search \
--mate-inner-dist 130 \
--library-type fr-unstranded \
$BOWTIEINDEX $READ1 $READ2

Following is the log file from Tophat run.

[2013-02-14 16:05:01] Beginning TopHat run (v2.0.6)
-----------------------------------------------
[2013-02-14 16:05:01] Checking for Bowtie
          Bowtie version:     0.12.7.0
[2013-02-14 16:05:01] Checking for Samtools
        Samtools version:     0.1.12.a
[2013-02-14 16:05:01] Checking for Bowtie index files
[2013-02-14 16:05:01] Checking for reference FASTA file
[2013-02-14 16:05:01] Generating SAM header for /app/references/iGenomes/homo_sapiens/hg19/UCSC/hg19/Sequence/BowtieIndex/genome
    format:         fastq
    quality scale:     phred33 (default)
[2013-02-14 16:05:24] Preparing reads
     left reads: min. length=101, max. length=101, 219973253 kept reads (259655 discarded)
    right reads: min. length=101, max. length=101, 219624658 kept reads (608250 discarded)
[2013-02-14 18:46:25] Mapping left_kept_reads to genome genome with Bowtie 
[2013-02-14 22:37:21] Mapping left_kept_reads_seg1 to genome genome with Bowtie (1/4)
[2013-02-14 23:39:33] Mapping left_kept_reads_seg2 to genome genome with Bowtie (2/4)
[2013-02-15 00:38:36] Mapping left_kept_reads_seg3 to genome genome with Bowtie (3/4)
[2013-02-15 01:41:39] Mapping left_kept_reads_seg4 to genome genome with Bowtie (4/4)
[2013-02-15 02:35:54] Mapping right_kept_reads to genome genome with Bowtie 
[2013-02-15 06:35:33] Mapping right_kept_reads_seg1 to genome genome with Bowtie (1/4)
[2013-02-15 07:32:53] Mapping right_kept_reads_seg2 to genome genome with Bowtie (2/4)
[2013-02-15 08:37:51] Mapping right_kept_reads_seg3 to genome genome with Bowtie (3/4)
[2013-02-15 09:43:46] Mapping right_kept_reads_seg4 to genome genome with Bowtie (4/4)
[2013-02-15 10:39:15] Searching for junctions via segment mapping
[2013-02-15 12:55:31] Retrieving sequences for splices
[2013-02-15 12:58:18] Indexing splices
[2013-02-15 13:19:49] Mapping left_kept_reads_seg1 to genome segment_juncs with Bowtie (1/4)
[2013-02-15 15:32:19] Mapping left_kept_reads_seg2 to genome segment_juncs with Bowtie (2/4)
[2013-02-15 17:49:12] Mapping left_kept_reads_seg3 to genome segment_juncs with Bowtie (3/4)
[2013-02-15 20:05:54] Mapping left_kept_reads_seg4 to genome segment_juncs with Bowtie (4/4)
[2013-02-15 22:14:28] Joining segment hits
    [FAILED]
Error running 'long_spanning_reads':Loading fusions...done

What could be the reason with this error ? I will greatly appreciate your help. Thanks !!

tophat fusion rna-seq sequencing mapping • 6.8k views
ADD COMMENT
0
Entering edit mode

What is your configuration (RAM) ?

ADD REPLY
0
Entering edit mode

I have 12GB of RAM.

ADD REPLY
1
Entering edit mode

I think the problem is there. Did you check the state of your process with top ? tophat with fusion-search and 200M reads used more than 12Gb I guess. Check the memory with top.

ADD REPLY
0
Entering edit mode

Thanks a lot. It was truly memory issue. I splitted FASTQ files into two and executed tophat fusion. It worked without reporting any error. Please post above comment as answer :D

ADD REPLY
1
Entering edit mode
11.8 years ago

I think the problem is there. Did you check the state of your process with top ? tophat with fusion-search and 200M reads used more than 12Gb I guess. Check the memory with top.

ADD COMMENT

Login before adding your answer.

Traffic: 2431 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6