Are you positive you're completely resuspending the beads? After my double digests, the BSA in the enzyme made it extremely sticky, and recovery was extremely difficult without extensive vortexing/centrifuging steps. You really need to make sure there's nothing stuck to the sidewalls of your well/tube, and that your bead/DNA mixture is quite homogeneous.

The problems were much less when I changed magnetic plates., and AmpureXP seems to much less sticky than the homemade variety.