1) I've done ddRAD, and a couple of other folks I know have also done ddRAD, and we just use standard desalting. The HPLC purification that is often recommended is considerably more expensive, and we've had good results without it.

Other methods of purification, like HPLC, make sure that nucleotides on the 5' end of an oligo aren't cut off during synthesis (rather, it makes sure that those that WERE cut short on the 5' end don't make it into the final product). That might be a consideration for T-overhangs that are used for the P2 adapter for RADseq (and might be less of a consideration for the longer overhangs in ddRAD). But others can chime in on that.

2) Why not just design your P2 adapter and primer after the Peterson et al. (2012) protocol? Literally the only thing you'd have to do differently is take their P2 adapter and change the sticky-end to append to an A-tail. Or am I missing some nuance here?

Thanks for your response. I had considered modifying the ddRAD P2 adapter; I just wanted to see what suggestions other people made.