AMPK Methods and Protocols

2.3 Specialist
Reagents
and Equipment

1. The protein purification protocol used here makes use of the
   A ̈KTA purification system (GE Healthcare). While these sys-
   tems are widely available in many laboratories, an alternative
   chromatography system or stand-alone peristaltic pump could
   be substituted.


2. Chromatography columns. Size exclusion chromatography,
   Superdex HiLoad prep grade XK 16/600 (GE Healthcare).
   Nickel affinity chromatography, HisTrap FF Sepharose, 5 mL
   (GE Healthcare).


3. For gel analysis of protein samples. The NuPAGE mini-gel
   system (Thermo Fisher Scientific) was used with 4–12% acryl-
   amide gradient Bis-Tris gels and the MES SDS gel running
   buffer system. The sample buffer was NuPAGE LDS sample
   buffer with 1 mM DTT. Mark12 markers (Thermo Fisher
   Scientific) were used to size the bands. InstantBlue (Expedeon)
   Coomassie protein stain was used to visualize the bands.


4. Protein was concentrated using Vivaspin protein concentrator
   columns (GE Healthcare).


5. The kinase CaMKKβwas prepared as described in Ref. [10].


6. The AMPK constructs were prepared in pET47 plasmid as
   described previously [4].


7. The benzimidazole derivative small molecule referred to as
   991 is an AMPK activator that binds at the ADaM site. 991 is
   used in this protocol to stabilize full-length AMPK for crystal-
   lization. Its chemical name is 5-[6-chloro-5-(1-methylindol-5-
   yl)-1H-benzimidazol-2-yl]oxy-2-methyl-benzoic acid, and it
   can be purchased as a custom synthesis from specialist chemical
   supplies such as SpiroChem AG. As 991 is sparingly soluble in
   aqueous solvents, a 10 mM solution in 100% dimethyl sulfox-
   ide (DMSO) needs to be prepared and stored at 20 C.


8. As an alternative to 991, the commercially available small mol-
   ecule ADaM-binding activator, A-769662 4-hydroxy-3-
   [4-(2-hydroxyphenyl)phenyl]-6-oxo-7H-thieno[2,3-b]pyri-
   dine-5-carbonitrile can be obtained from ApexBio Technology.
   Crystals obtained with this ligand diffract less well possibly due
   to the lower affinity of A-769662 compared to 991.

3 Methods

3.1 General Points The first part of the protocol below describes optimized methods
for expression and purification of crystallization-grade full-length
AMPKα 1 β 1 γ1; however, the protocol can equally be used to
produce the truncated core domain AMPK, which has also been
crystallized [2]. Full-length protein is prone to aggregation during
this process. This has been reduced by optimization of the process

4 Julia A. Hubbard et al.