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Hi all!
We are trying to use Dindel for generating re-aligned .bams from Illumina PE-read data. I was able to run through the Dindel pipeline, but noticed that in the output .sam files (generated following the instructions given in Dindel manual), many reads were output more than once.
When examining my data, I realized that overlapping windows were created in Dindel Stage 2. (The makeWindows.py step.) This is probably the reason why I was getting multiple reads in the concatenated .sam files.
Has anyone else encountered the same problems while attempting to get re-aligned .bam files? Do you know any solutions? Merging windows would be an obvious option, but could this result in large windows with unmanageable number of distinct haplotypes?
Any comments are welcome! 8)
Yilong
We are trying to use Dindel for generating re-aligned .bams from Illumina PE-read data. I was able to run through the Dindel pipeline, but noticed that in the output .sam files (generated following the instructions given in Dindel manual), many reads were output more than once.
When examining my data, I realized that overlapping windows were created in Dindel Stage 2. (The makeWindows.py step.) This is probably the reason why I was getting multiple reads in the concatenated .sam files.
Has anyone else encountered the same problems while attempting to get re-aligned .bam files? Do you know any solutions? Merging windows would be an obvious option, but could this result in large windows with unmanageable number of distinct haplotypes?
Any comments are welcome! 8)
Yilong
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