I aligned RNA-Seq reads to the reference genome. However, reads that span splice junctions will not align. What is the best way to handle this? I've read that aligning to a reference transcriptome is not the answer. Any thoughts? Thanks!
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You might want to try TopHat/Bowtie.
Alternatively, you can download all mRNA sequences from UCSC and align against that.
Sam
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So I used tophat 2 to align the data. I used multiple cores but ran it on the default settings.
I have tumor and normal samples (no replicates, single end).
My accepted_hits.bam for the normal samples is 479MB while the unmapped.bam file is 3.4 GB. I was wondering what I might be able to do about this? I am re-aligning the unaligned reads in BWA, but I'm not sure if this is the best approach. Any thoughts? There should not be so few mapped reads for this sample. The tumor samples had an unmapped.bam file of size 796 MB and an accepted_hits.bam file of size 479 MB. Although this is better, it still seems low.
The normals should actually be better than the tumors due to sample quality.
Thanks in advance for your help!
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Did you quality trim before running the alignment? If not and a lot of your reads deteriorated in quality toward the end, that could be the issue. You might also try blasting a couple of the unmapped reads just to ensure there's nothing weird going on.
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