Western Blotting Protocol 

Buffers:

TBS:  25 ml of 1 M Tris-7.5, 30 ml of 5 M NaCl, bring volume up to 1000 ml with ddwater

TBS-T:  TBS + 0.5 ml of Tween 20

5X SDS-PAGE running buffer:  15.1 g Tris base, 94 g glycine in 900 ml water, then add 50 ml of 10% solution of SDS, and adjust volume to 1000 ml with ddwater

Blocking solution:  5 g nonfat dry milk in 100 ml of PBS

Transfer Buffer:  5.82 g Tris base + 2.93 g glycine + 0.375 g SDS (or 3.75 ml of a 10% solution of SDS) + 200 ml methanol, then bring volume up to 1 liter with ddwater

Prepare cell extracts using an appropriate protocol. 

7.     Block in 75 ml of blocking solution overnight at 4 C (alternatively, block at room temp for 1 h on a shaking platform).

8.     Wash 3 times with TBS-T, each for 10 min.

9.     Make dilution of primary antibody (usually 2 ul in 10 ml of TBS), and add to membrane, shake on a platform for 1 h at room temp.  Make sure that membrane is entirely covered with antibody solution.

10.  Discard antibody solution and wash with TBS-T 3 times for 10 min each.

11.  Make dilution of secondary antibody (usually 1 ul in 10 ml), and cover membrane with antibody solution and shake on a platform for 1 h at room temp.

12.  Discard antibody solution, and wash membrane with TBS-T 4 times for 10 min. each.

13.  Detection using the ECL/ECLplus kit