AMPK Methods and Protocols

14. Open the abdomen to expose the organs in the peritoneal
    cavity and tightly clamp the edge of liver with the prefreezed
    clamp for 20 s.


15. Homogenate some 50 mg of frozen liver using an
    electrical disperser in 1 mL of methanol containing IS1
    (1:200;seeNote 41).


16. Extract ATP, ADP, and AMP as described insteps 4– 11 of
    Subheading3.4.

Measure the Levels of AMP, ADP, and ATP Using CE-MS

17. Maintain the fused-silica capillary at 20C prior to use (see
    Note 42).


18. Couple CE unit with TOF-MS unit by passing the sheath
    liquid through the coaxial sheath at 10μL/min for 30 min.


19. Run CE-TOF-MS at anion mode and analyze the levels of
    adenylates. In detail, the fused-silica capillary is first filled
    with ammonium acetate solution and then preconditioned
    with the electrolyte containing phosphate buffer. At the begin-
    ning of each run, the capillary is washed by electrolyte contain-
    ing phosphate buffer. Sample is injected by Agilent 1100 series
    pump at a pressure of 50 mbar for 25 s and is driven by a
    constant voltage at 30 kV (for 40 min). The fragmentor volt-
    age of MS unit at three directions is set at 125, 50, and 650 V,
    respectively. The voltage for ionization is set at 3500 V, with a
    drying gas flow at 7 L/min at 300C. The separation is assisted
    by a nebulizer at 15 mbar pressure. The isotope of the depro-
    tonated acetic acid (m/z60.0172) and 2,2-difluoromethoxy
    phosphazene plus deprotonated acetic acid (m/z680.03554)
    are used as the reference masses. The scanning range is
    50–1000m/z, and the scan rate is 1.5 spectra/s.

4 Notes

1. Dialysis of FBS is not necessary, since the glucose brought by
   10% (v/v) FBS is not sufficient to affect the activation of AMPK
   under glucose starvation.
   2.LAMTOR1
   /
   orAXIN
   /
   MEFs are generated by infecting
   SV40 T-immortalizedLAMTOR1F/ForAXINF/FMEFs with
   adenovirus expressing Cre recombinase for 12 h. To avoid the
   elevated basal levels of p-Thr-172-AMPKαin the infected cells,
   we strongly recommend that cells be incubated in fresh
   DMEM for another 8–10 h before further treatments.


2. According to our experience, the genomes ofLAMTOR1
   /
   
   MEFs are unstable. We therefore recommend generating
   knockout MEFs fresh for each experiment.

406 Chen-Song Zhang et al.