AMPK Methods and Protocols

buffer for each sample. This minimizes the time the muscle is at

4 C where enzymatic processes slowly start up. Once the tissue

is lysed, the proteins and enzymes are extracted and mixed with

protease and phosphatase inhibitors, and then the time pres-

sure for having the sample at 4C is lowered.

5. The Protein A or G agarose is usually supplied in a suspension
   containing ethanol and has to be calibrated in the IP buffer.
   When pipetting the agarose, use wide orifice pipette tips and
   vortex or stir the suspension just before pipetting.


6. The Pre-IP is the same as the input material to the IP procedure
   and could be the raw lysate. Mixing the lysate with agarose
   beads and antibody and incubating it overnight could however
   make small changes in the appearance of protein bands on a
   SDS-polyacrylamide gel (also proteins not precipitated). To
   make the best comparison between Pre- and Post-IP, a control
   IP with an unspecific/irrelevant antibody should be made, and
   the Post-IP of this should be used as Pre-IP (input).


7. The amount of antibody to be used in an IP depends on the
   amount of lysate precipitated on and the affinity of the anti-
   body, which must be tested. Usually 2μg of antibody is suffi-
   cient for IP on 200μg of lysate. The concentration of antibody
   varies between batches, and also to avoid pipetting very small
   volumes, it is recommended to dilute the antibody in IP buffer
   to a concentration of 0.2 mg/ml and then pipette 10μlto
   each IP.


8. The amount of lysate protein put into the IP depends on the
   purpose of the IP. Searching for co-IP of AMPK heterotrimeric
   complex partners, the IP and Post-IP must be used for several
   Western blots detecting all seven subunit isoforms. The
   amount of protein loaded on gels for these blots depends on
   the antibodies used for the blots, but are in the range of
   5–20μg, and some isoforms with different molecular weight
   can even be analyzed on the same gel. Precipitating on 200μg
   of lysate protein would give material enough for loading at least
   five gels.


9. The time and temperature for an IP can vary a lot depending on
   antibody affinity, considerations for protein complex stability,
   and workflow. Low temperature (4C) lengthens the IP pro-
   cess, but maintains a higher stability for protease and phospha-
   tase inhibitors as well as for protein interactions. Doing
   consecutive IPs and measuring enzyme activity on each of the
   IPs would challenge the number of hours in a working day if
   the time for each IP was set to only a couple of hours. Our
   experience is that the AMPK heterotrimeric complexes are very
   stable and can endure at least three consecutive overnight IP
   incubations at 4C.

Analysis of Heterotrimeric Complex Stoichiometry 211