Protein Extraction for Amyloid Beta Fractionation

5x Homogenization Buffer (store 4oC): ^oC):

125 ml of 1.0 M Tris

30 ml of 0.5 M MgCl₂

25 ml of 0.1 M EDTA (pH to 7.2 and store at 4°C for up to 6 months)

20ml of MiliQ Water

1x Homogenization Buffer (dilute day of):

Dilute 5x Homogenization buffer to 1x in MiliQ Water and add 1 tablet protease inhibitor (cat#11697498001 Roche) per 10 mL

1x Homogenization Buffer with 1% Triton X (dilute day of):

Add 1% Triton X-100 to 1x Homogenization buffer made above

70% Formic Acid (store RT) Caution Acidic

7mL formic acid

3mL water

1.5x Homogenization Buffer pH 14 (store 4oC) ^oC) Caution Corrosive

Dilute 5x Homogenization buffer to 1.5x in MiliQ Water and pH to 14

Weigh frozen tissue sample and record for later normalization

Homogenize the tissue on ice using quick bursts of a sonicator in 400µl 1x Homogenization buffer

Centrifuge maximum speed at 4°C for 1hr

Collect supernatant as tris soluble fraction and store -80°C for later use

Homogenize the pellet on ice using quick bursts of a sonicator in 200µl 1x Homogenization Buffer with 1% Triton X-100

Centrifuge maximum speed at 4°C for 1hr

Collect supernatant as triton soluble fraction and store -80°C for later use

Homogenize the pellet on ice using quick bursts of a sonicator in 50µl 70% formic acid Be careful with acid

Centrifuge maximum speed at 4°C for 1hr

Collect supernatant as formic acid soluble fraction and neutralize with 1.5x Homogenization buffer pH14 on ice Be careful with acid and base*. Store -80°C for later use