In paired-end sequencing fragment libraries are sequenced from termini of insert. The reads not only provide coverage but also provides distance information which can be useful in many applications such as de novo assembly and identifying structural variation. In Illumina systems cost per base or read for 2nd reads is less than single end read. Contigs from short reads cannot be assembled in repeat regions and collapse. In these cases mate pair libraries larger than repeat region size are particularly useful for orienting and ordering contigs relative to each other. Mate pair libraries usually are constructed by circularising long fragments (2-20 kb), shearing and capturing the termini junction followed by library prep and paired-end sequencing.

Thank you for the information.

Jayakumar S