AMPK Methods and Protocols

6. Dilute 30μg of total protein with lysis buffer to 15μl of total
   volume, mixed with 5μlof4loading buffer, and heat at
   95 C for 5 min. Afterward the samples can be stored at
    20 C until further analysis by SDS-PAGE (seeSubheading
   3.5)(seeNote 27).

3.5 SDS
Polyacrylamide Gel
Electrophoresis
and Immunoblotting

1. For a 7.5% SDS polyacrylamide gel, mix 5 ml of H 2 O, 2.5 ml of
   polyacrylamide solution, and 2.5 ml of resolving gel buffer (see
   Note 28). For a 15% SDS polyacrylamide gel, mix 2.5 ml of
   H 2 O, 5 ml of polyacrylamide solution, and 2.5 ml of resolving
   gel buffer (seeNote 29). Start polymerization by adding 65μl
   of APS and 15μl of TEMED.


2. The 5% stacking gel consists of 3.125 ml of H 2 O, 1.25 ml of
   stacking gel buffer, and 0.625 ml of polyacrylamide solution.
   To start the polymerization, add 25μl of APS and 8μlof
   TEMED.


3. Load the samples from Subheading3.4 onto a 7.5% or a 15%
   SDS gel and separate electrophoretically at 150 V for about
   1.5 h until the bromophenol dye front just ran off the gel (see
   Notes 3and 27 ).


4. Blot the 15% SDS gels with the semidry method. Equilibrate
   six Whatman filter papers, a nitrocellulose membrane, and the
   SDS gel for a few minutes with semidry transfer buffer. After-
   ward stack them on the semidry blotting apparatus in the
   following order starting from the cathode: three filter papers,
   SDS gel, nitrocellulose membrane, and three filter papers.
   Perform the transfer at 1.9 mA per cm^2 of nitrocellulose mem-
   brane for 1.25 h and maximal 40 V.


5. Blot the 7.5% SDS gels with the wet blotting method. Equili-
   brate two sponges, six Whatman filter papers, a nitrocellulose
   membrane, and the SDS gel in ice-cold tank blot transfer buffer
   for a few minutes. Afterward stack the holder cassette inside the
   container with the black side facing down in the following
   order: a sponge, three filter papers, SDS gel, nitrocellulose
   membrane, three filter papers, and a sponge. To remove bub-
   bles from the stack, use a glass pipette and roll over it carefully.
   Close the holder cassette carefully in the container, and place
   into the blotting chamber with the black side facing black and
   the white side facing red. Place the cooling unit inside the
   chamber as well, and fill it up with ice-cold tank blot transfer
   buffer. Run the tank blot at 100 V for 1 h.


6. After the transfer, incubate the blots with IB blocking solution
   for at least 1 h at room temperature on a horizontal shaker.


7. Subsequently wash the blocked blots several times in TBS-T
   (seeNote 30) until the incubation with primary antibody at
   4 C overnight on a rocking device (seeNote 2).

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