The preferred substrate for Degradase and Degradase Plus is double stranded DNA. There will be only minor degradation of single stranded DNA template and no degradation of RNA template.

Yes, you can scale the reaction up or down as necessary. For the best results, digest no more than 1µg of DNA with 5U (1µl) of enzyme in 25µl reaction volume. The reaction volume is just as important as the amount of DNA, and we recommend scaling up the volume of enzyme accordingly. For example, if the reaction volume is 100µl, use 4µl of DNA Degradase (Plus).

Yes, the protocol time is a suggestion for sufficient digestion. Additional incubation time can be added to completely ensure that all sample has been digested. There is no harm in letting the reaction proceed longer.

Yes, you can add excess enzyme to ensure full digestion.

The best way to confirm degradation is to run the sample on a gel. Nothing should be visible for the Degradase-treated samples. You do not need to purify the reaction.