You are ready to set up your reaction.  You are provided with a stock of plasmid DNA that is at a concentration of 1mg/ml.  You have stock enzyme buffer that is 10X (meaning it is ten-times more concentrated than you need it to be in the actual reaction).  You have deionized water (dH₂O) to use, as needed.

• How many ml of DNA will you add to your reaction tube?
• How many ml of 10X buffer will you add to your reaction tube?
• How many ml of  ApeKI will you add to your reaction tube?
• How many ml of dH₂O will you add to your reaction tube?
• At what temperature will you incubate the reaction?

So how would you solve for these?