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I am using 100 bp paired end Illumina Hi-seq data with about 50M reads and trying to use tophat / cufflinks for RNA-seq analysis for human data, using Ensemble v68 gtf along with Gencode v13 lncRNA gtf annotations. These files were concatenated together to run both tophat 2.0.6 with bowtie2 2.0.6:
tophat -p 4 --solexa1.3-quals --read-realign-edit-dist 0 --no-novel-juncs --library-type fr-unstranded -G $GTF -o $OUT $GENOME $FASTQ_1 $FASTQ_2
and Cufflinks 2.0.2
cufflinks -o $OUT -p 4 -G $GTF -b $FASTA --multi-read-correct $OUT/accepted_hits.bam
A segmentation fault has continued to occur with multiple samples at similar locations as Cufflinks is re-estimating abundacnes with bias and multi-read correction. Below is the output:
[09:41:21] Learning bias parameters.
> Processed 635 loci. [*************************] 100%
[09:45:58] Re-estimating abundances with bias and multi-read correction.
> Processing Locus chr16:5289802-6826015 [******* ] 31%Segmentation fault (core dumped)
Any input would be greatly appreciated.
tophat -p 4 --solexa1.3-quals --read-realign-edit-dist 0 --no-novel-juncs --library-type fr-unstranded -G $GTF -o $OUT $GENOME $FASTQ_1 $FASTQ_2
and Cufflinks 2.0.2
cufflinks -o $OUT -p 4 -G $GTF -b $FASTA --multi-read-correct $OUT/accepted_hits.bam
A segmentation fault has continued to occur with multiple samples at similar locations as Cufflinks is re-estimating abundacnes with bias and multi-read correction. Below is the output:
[09:41:21] Learning bias parameters.
> Processed 635 loci. [*************************] 100%
[09:45:58] Re-estimating abundances with bias and multi-read correction.
> Processing Locus chr16:5289802-6826015 [******* ] 31%Segmentation fault (core dumped)
Any input would be greatly appreciated.
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