Hi,

the extra peak is probably due to overamplification which can give you ssDNA that migrates slower than dsDNA. See e.g. slide 30 here: http://www.mbl.edu/jbpc/files/2014/0..._slideshow.pdf

Well, probably not completely ssDNA.

If the PCR reaction runs low on primers and high on products, then amplicons annealing back to each other becomes kinetically favorable. But since this is a library then the likelihood is that the inserts of the two annealling amplicons will be unrelated. So you end up with "bubble" products. Double-stranded at the ends (where the adapters are) but with little or no annealing in the middle.

These floppy bubble products apparently migrate slowly and so appear to be larger than they actually are. Happily you can pretty much ignore them as they cluster and sequence fine. (Although they can play havoc with your cluster titrations if you don't understand what they are.)

This probably the single most common artifact posted to this forum! But in recent years one only sees new posts about it a couple of times per year.

--
Phillip

The Illumina Truseq protocol must be written horribly - almost all of our customers using the Truseq RNA-seq kit for the first time totally over-amplify their libraries (15 cycles).