Bowtie 2 error- bowtie2-align died with signal 6 (ABRT): Help please!
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2.1 years ago
sayema.khan ▴ 10

Hi all, I am looking to map my pair-ended trimmed reads to my reference genome using Bowtie2. I input the R1 and R2 fastq files and the reference genome FASTA file. It gives me the below error and I am not sure how to fix this.

Error, fewer reads in file specified with -2 than in file specified with -1 Error, fewer reads in file specified with -2 Error, fewer reads in file specified with -2 than in file specified with -1 than in file specified with -1 Error, fewer reads in file specified with -2 than in file specified with -1 Error, fewer reads in file specified with -2 than in file specified with -1Error, fewer reads in file specified with -2 than in file specified with -1

Error, fewer reads in file specified with -2 than in file specified with -1 Error, fewer reads in file specified with -2 than in file specified with -1 terminate called after throwing an instance of 'int' terminate called recursively terminate called recursively (ERR): bowtie2-align died with signal 6 (ABRT)

The R1 and R2 reads are definitely same size and I also have enough space left on my galaxy for analysis.

Any help much appreciated on how I can fix this please?

chipseq Bowtie2 mapping • 948 views
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Have you trimmed these files and not used paired-end mode eventually?

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Hi! Have you tried to count the number of reads in each file? You could try some of the answers suggested at How to count fastq reads.

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Size is not an indicator for number of reads. Did you process these reads somehow, like trimming? A common rookie mistake is trimming PE data with a non-PE trimmer, causing unsynced files.

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