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BQ-042-101-05
Revision : 2 (2016-07-04)
f. DNA Clean-Up
1.
Transfer the eluate or enzyme reaction product to each specific tube format.
a. (Mini) Transfer the eluate to a 1.5 ml or 2 ml tube
b. (Midi/Maxi) Transfer the eluate to a 15 ml tube
2.
If RNA-free genomic DNA is required, add up to 10 μl (mini)/ 75 μl (midi)/ 150 μl (maxi) of RNase A
(see “Before you begin”) and incubate for 2 min at room temperature.
3.
(Binding)
Add 1 volume of Buffer ② (Binding) to the eluate and mix completely by vortex mixer.
4.
(DNA precipitation)
Add 3 volumes of absolute ethanol to the eluate and mix well by vortex mixer.
5.
(DNA binding with Magnetic Nano Bead: 5-7)
Add 100 μl (mini)/ 500 μl (midi)/ 1 ml (maxi) of Magnetic
Nano Bead solution
to the tube and mix thoroughly using a vortex mixer until the beads are fully
resuspended.
(Note) Magnetic Nano Bead
Solution contains magnetic nano beads. Please shake well before use.
6.
Place the tube in
MagListo™-2 (mini)/ MagListo™-15 (midi, maxi) Magnetic Separation Rack with the
magnet plate attached and invert the tube 3~4 times gently until the beads tightly bind to magnet.
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Attachment
Combine the magnet plate to the stand.
7.
Without removing the tube from
MagListo™ rack, carefully pour the supernatant out and completely
remove the remaining supernatant using paper towel by blotting.
