I'm also curious about this. Whatever they use, it's likely very important that the polymerase has very low strand displacement activity and NO 5'=>3' exonuclease activity. I suspect the ligase is not thermostabile, given that the on column ligation takes place at 37C (taq ligase is active at 45-65), although the NaOH they use during elution surely inactivates both the polymerase and ligase.

My curiosity is whether these steps can be performed in the absence of any pre or post column purification. A solution that hybridizes, extends, and ligates in a linear but cycle-able way would be ideal. If enough copies of the desired ligated product can be generated, it's possible that dilution could be used to carry the product into direct barcoding PCR, rather than purification. Anyone tried anything like this?