Hi everyone!

I have been using CIRCexplorer2 in single-end RNA sequencing datasets for a while, however, I have never use it for paired end data. In the papers and suplementary methods of circexplorer and circexplorer2 it is clearly explained how does the program identify circRNA in single-end datasets. It aims to identify the backspliced junction read of the circRNA, that's it, a read that maps in a non-colinear order to the genome.

However, for paired end datasets, using tophat-tophat-fusion, I think that there could be different aproaches to identify circRNA, as one could have, different indicators for circRNAs, for example:

• The left reads with the backsplicing read and the right read mapping to an exon.
• The right part of the read will map in the genome before the left part

Does anyone know how does CIRCexplorer2 adress this problems?

Thanks for reading,

The latest version of CIRCexplorer2 has supported paired end datasets. See http://circexplorer2.readthedocs.io/en/latest/tutorial/alignment/ for details.