You could use non-standard synthesis http://onlinelibrary.wiley.com/doi/1....nc0434s36/pdf...

I thought I had read that phosphorothioate linkages, while resistant to many exonucleases, were not resistant to T4 polymerase. If so, then the phophorothioate linkage will be of limited utility. After "end polishing + A-tailing" there is an Ampure clean up. This will likely remove the majority of exonucleases contaminating the original DNA prep. If any nuclease were to remain, one would think it would be the one that is deliberately added during "polishing" -- T4 polymerase. Or is T4 poly not used to remove 3' overhangs in the TruSeq kit?

--
Phillip

Thanks Phillip,

I won't be doing that synthesis! (but thanks). There are two exonucleases that cause problems. One comes along with the ligase in the adapter ligation step (I don't know if it's intrinsic to the ligase itself or just a contaminant). So the 3' T-tail on the duplex end of the adapter is linked with phosphorothioate, to prevent adapter dimer formation (perhaps less of a problem for mate pair libs that are cleaned up with streptavidin beads (the free adapter get washed away). The second exonuclease is part of the proofreading activity of the Finnzymes Phusion polymerase used in library amplification. I can't avoid that one either. So my PCR primers have a 3'-terminal phosphorothioate linkage. These primers do get chewed during PCR and it is causing some problems. Thanks again.

hi memri, are you sure they are treating with exonuclease? sounds like an unnecessary extra step ?

For the PCR, yes. For the ligation, probably not.

Yow! Are you talking about the PPC (PCR Primer Cocktail) from the TruSeq kits? I don't know what is going on with them. Take a look at this. They run at 80-85 nt! Makes no sense...

--
Phillip