AMPK Methods and Protocols

lasting approximately 7 days. It is mandatory to daily check the

food intake and body weight.

6. The specificity of dissection can be tested by detection of
   contamination from adjacent nuclei by measurement of specific
   markers of each nucleus, such as steroidogenic factor-1 (SF1) as
   a marker of the VMH, proopiomelanocortin (POMC) for the
   ARC, or orexin for the LHA. Analysis should be carried by
   RT-PCR [40]


7. For the whole hypothalamus (rat/mouse), use 400/200μL
   BLYSpi, while for a nucleus-specific dissection, use
   200/100μLBLYSpi.


8. Increase time if necessary. It is very important to complete the
   disaggregation of the tissue in order to achieve a high protein
   concentration. With low volumes of BLYSpi, some foam may
   form. Centrifuge the tubes for 10 s at maximum speed in a
   benchtop centrifuge. You should be able to see the clear
   homogenate with no bubbles. We recommend using safe-lock
   tubes.


9. It is recommended putting all tubes in the same orientation
   into the centrifuge. This way it is possible to know the position
   of the pellet in the tube even if it is not possible to see it.


10. If the protein concentration is too low, it is possible to increase
    the final volume of the loading, i.e., without altering the
    amount of protein loaded to the gel.


11. During the electrophoresis, the migration front can fade. This
    may be due to a change in the pH of buffers or to abrupt
    temperature changes.


12. Do not let the filter paper or the membranes become dry. Wet
    with more transfer buffer 1when necessary.


13. Avoid using milk-based blocking since it may contain
    phosphatases.


14. To detect changes in the phosphorylation of AMPKα at
    Thr-172, we use a Cell Signaling Technology antibody (rabbit
    monoclonal anti-phospho-AMPKα (Thr-172), Cat#2535S)
    diluted 1:2000 for total hypothalamic (20μg of protein per
    sample) detection or 1:1000 (10μg of protein per sample) for
    nucleus-specific detection. pAMPK is normalized withβ-actin
    protein levels, although AMPKα1 and AMPKα2 (or total-
    AMPK) levels should always be displayed. To detect the levels
    of AMPKα1 and AMPKα2, we use Merck Millipore antibodies
    (rabbit polyclonal anti-AMPKα1 and anti-AMPKα2, Refs
    07-350 and 07-363, respectively) diluted 1:1000. To detect
    the total levels of AMPKα, we use a Cell Signaling Technology
    antibody (rabbit polyclonal anti-AMPKα, Cat#2532) diluted
    1:1000.

Methods for Brain AMPK 445