AMPK Methods and Protocols

10. The 6SB should comprise a sixth of the total volume in a
    sample made ready for SDS-PAGE. 170μl Post-IP/5¼ 34 μl.


11. Leave a small volume (190–170¼ 20 μl) of the supernatant
    with the IP to minimize the risk of transferring agarose beads
    to the Post-IP. This small amount of supernatant is washed
    away afterward. The Post-IP can be used for several Western
    blots detecting the presence (not coprecipitated) or absence
    (coprecipitated) of different subunit isoforms and other
    proteins.


12. If the specific protein was precipitated from 200μg of lysate
    protein and all of the specific protein was precipitated success-
    fully, then adding 20μlof2SB to the agarose beads would
    give a protein concentration corresponding to 10 mg/ml. This
    is not the real protein concentration, but the amount of the
    specific precipitated protein would be equivalent to that in
    20 μl of lysate with a total protein concentration of 10 mg/ml.


13. The amount of lysate protein to be put into the IP and the
    volume of the IP are adjustable as one finds suitable. Increasing
    the amount of protein and/or decreasing the volume gives a
    higher protein concentration in the Post-IP. The volume
    should be sufficient to allow for proper fluid mixing in the
    tube during the IP end-over-end incubation. Smaller tubes
    (0.2 ml PCR tubes) are suitable for smaller IP volumes.


14. Since the IP only contains a “few” proteins (the precipitated
    and coprecipitated proteins, plus the antibody and the protein
    G from the agarose) compared to a lysate, it will often behave
    differently on SDS-PAGE. Occasionally the specific protein
    band shifts upward in molecular weight and does not align
    with the band in the Pre-IP. Furthermore, when loading the
    same amount of protein based on the input to the immuno-
    precipitation, the signal intensity of the IP band is different
    from the corresponding band from the Pre-IP. Often the West-
    ern blot signal in the IP is lower with the exception of theγ 1
    isoform, which is stronger. It is therefore advisable to load
    twice the amount of protein from the IP compared to the
    Pre- and Post-IPs to get similar signal intensity on the Western
    blot. However, due to these and other circumstances men-
    tioned above,do not quantitatively compare IP signals to the
    signals of the Pre- and Post-IPs.

References

1. Stapleton D, Mitchelhill KI, Gao G, Widmer J,
   Michell BJ, Teh T, House CM, Fernandez CS,
   Cox T, Witters LA, Kemp BE (1996) Mamma-
   lian AMP-activated protein kinase subfamily. J
   Biol Chem 271:611–614
   2. Mahlapuu M, Johansson C, Lindgren K,
   Hjalm G, Barnes BR, Krook A, Zierath JR,
   Andersson L, Marklund S (2004) Expression
   profiling of the gamma-subunit isoforms of
   AMP-activated protein kinase suggests a major

212 Jesper B. Birk and Jørgen F. P. Wojtaszewski