Foreskin Tissue DNA Extraction

Add steel bead to 1.5 ml tube

Add 800 µL CD1 to tube

Weigh tube (with bead and solution)

Dissect approximately 25 mg (3 mm³) piece of tissue

Fragment tissue with scalpel

Add tissue to tube (with bead and solution)

Weigh tube and calculate net tissue weight.

Process tubes on TissueLyzer II, 2 min at 30 Hz

Rotate block 180º and repeat

Centrifuge tubes briefly to collapse foam

Spin PowerBead Pro plate to ensure beads are settled at the bottom

Add contents of each specimen tube (except steel bead) to a PowerBead plate well

Add 5 µL of 20 mg/ml proteinase K to each well

Seal plate with film

Vortex briefly to mix

Incubate plate at 65º C for 60 min or until tissue is mostly digested

Process plate on TissueLyser II, 5 min at 25 Hz

Rotate plate 180º and repeat

Centrifuge plate at 3000 x g for 7.5 min

Transfer approximately 350 µL supernatant from each well to fresh S-block using well-vator

add 300 µL of solution CD2 to each well and mix thoroughly by pipetting

Seal the plate with film

Centrifuge at 3000 x g for 7.5 min at room temperature

Avoiding the pellet, transfer 500 µL of supernatant to fresh S-block using well-vator

Follow DNeasy 96 PowerSoil Pro Protocol for QIAcube HT (page 17 onward)

Elute in maximum volume (120 µL)

Incude vacuum performance check

Seal plate and freeze at -20ºC