Anchor Binding Capacity

What you will need:

Make a series of 50 μL serial dilutions of 2 μM Anchor solution (1/2, 1/5, 1/10, 1/15, 1/20, 1/25, 1/30, etc)
Prepare a tube for each dilution of Anchor made, each containing 40 μL 4 mg mL^-1 beads.
Wash the beads twice with 100 μL Wash/Binding buffer and once with 100 μL water, then aspirate water off the beads.
Add 20 μL of each dilution to it's respective tube with washed beads.
Let bind at room temperature for 10 minutes.
Take readings at A₂₆₀ with a UV-Vis Spectrophotometer of the dilutions prior to binding to bead and after binding to bead. (ng of DNA can also be found by in-gel band intensity quantification methods)
Convert DNA measurements to pmol and plot pmol DNA versus mg of beads. The slope gives the binding capacity