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Hello all,
I am aligning paired-end reads using Hisat2. Unfortunately, some of the fastq files were corrupted in transfer. I was able to recover them using a gzip recovery protocol, but was left with about half the data. I have previously used Tophat2 to align these "recovered" fastq files, but am getting this error when trying to align with Hisat2:
How is Tophat2 dealing with this differently than Hisat2?
To fix this, I am trying repair.sh from the bbtools package to keep the reads that do have pairs in both files and output singletons to a seperate file and then try using all three with Hisat2.
Although I can't seem to find reference to this error anywhere else, any advice on how I should deal with this?
I am aligning paired-end reads using Hisat2. Unfortunately, some of the fastq files were corrupted in transfer. I was able to recover them using a gzip recovery protocol, but was left with about half the data. I have previously used Tophat2 to align these "recovered" fastq files, but am getting this error when trying to align with Hisat2:
Code:
Error, fewer reads in file specified with -2 than in file specified with -1
To fix this, I am trying repair.sh from the bbtools package to keep the reads that do have pairs in both files and output singletons to a seperate file and then try using all three with Hisat2.
Although I can't seem to find reference to this error anywhere else, any advice on how I should deal with this?
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