Hello,

I downloaded a bunch of RNA-seq dataset from Genbank and used tophat (with Bowtie2) to map back to the genome (to create a gtf file). The data are paired-end.

Out of the 5 samples, three of them gave a strange alignment result. The right read would realign 90% of the reads BUT only 0.3% of the left reads. Obviously, I downloaded the data 3 times, made sure it was not an error from my end.

So something is wrong with the left reads, using bowtie I can realign single end with 90% for both files, and 60% on paired end data. But tophat would only work for the right reads with paired end.

I was wondering if you had any ideas what could be causing the problem, I would like to contact the authors but with a good explanation of what the issue could be.

Thanks for your help

First, I'd check the raw-data with FastQC in order to control for low-quality tails and adapter contamination.

Second, I'd check the inner-distance with a subset of reads (aligning with bowtie2 and RSeQC's inner_distance.py). You should adjust the Tophat's --mate-inner-dist and --mate-std-dev parameters. Tophat is trying to learn the inner distance distribution, but providing theses data increases accuracy.

Take a look the type of library setting in the analysis. I refer to the --library-type setting.