Blue Native Gel Electrophoresis
Stock solutions
49.5%T, 3%C Acrylamide
24 g acrylamide, 0.75 g
bisacrylamide / 50 ml H2O
Store at RT
3 x Gel buffer
150 mM BisTris-HCl, 1.5 M
6-amino-caproic acid, pH 7.0
Adjust pH to 7.0 with HCl at 4°C
Store at 4°C
75% (w/v) Glycerol
Store at 4°C
10 x Cathode buffer
0.5 M Tricine, 150 mM BisTris
No need to adjust pH
Store at 4°C
5 x Anode buffer
0.25 M BisTris-HCl, pH 7.0
Adjust pH to 7.0 with HCl at 4°C
Store at 4°C
2 x BisTrisACA
200 mM BisTris-HCl, 1 M
6-amino-caproic acid, pH 7.0
Adjust pH to 7.0 with HCl at 4°C
Store at 4°C
50BTH40G
50 mM BisTris-HCl,
40% (w/v) Glycerol, pH 7.0
Adjust pH to 7.0 with HCl at 4°C
Store at 4°C
Working solutions
1xCathode (-dye), 1x Anode
buffer
Store at 4°C
1xCathode+dye
0.01% Serva G in 1xCathode buffer
It takes a while to dissolve
ServaG.
Store at 4°C
BN-sample buffer
|
Serva G |
50 mg |
|
2 x BisTrisACA |
500 ul |
|
75% Sucrose |
400 ul |
|
H2O |
100 ul |
Store at -20°C
Solubilization buffer
|
50BTH40G |
100 ul |
|
10% Detergent |
40 ul |
|
H2O |
60 ul |
§ Detergent: TX-100, dodecyl-maltoside, digitonin or SDS
§ Water soluble digitonin should be used.
§ If you don’t get water-soluble digitonin, purify as described in Mori et al. (1999) J Cell Biol. 146, 45-55. We've also tried 2X crystalized digitonin with essentially the same results.
§ Note: the original method uses ACA in the solubilization buffer.
5-13.5% gradient blue native gel
Mini gel with 0.75 mm spacer
|
|
Sample
(4%) |
Separation |
Separation |
|
49.5% Acrylamide |
0.242 ml |
0.212 ml |
0.573 ml |
|
3 x Gel buffer |
1.0 ml |
0.7 ml |
0.7 ml |
|
75% Glycerol |
0 |
0.14 ml |
0.56 ml |
|
H2O |
1.72 ml |
1.028 ml |
0.247 ml |
|
TEMED |
6 ul |
2 ul |
2 ul |
|
5% AP Pour into a gradient maker |
32 ul |
11 ul 1.88 ml |
11 ul 1.8 ml |
|
Total |
3.0 ml |
2.1 ml |
2.1 ml |
- Use mini alumina and glass plates
- Sample gel height should be ~0.7 cm
- Make gel one day before use and store at 4°C
Sample preparation
Wash thylakoids with 0.33 M
Sorbitol, 50 mM BisTris-HCl, pH 7.0
Resuspend in 25 mM BisTris-HCl, 20% Glycerol, pH 7.0
Adjust [chl] to 2.0 mg/ml (or resuspend thylakoids in the resuspension buffer
to 2.0 mg chl/ml)
Add one volume of solubilization buffer, gently vortexing after each drop
Agitate for 30 min (DM, TX-100), 30-60 min (Digitonin) at 0 to 4°C
Spin at ~100,000 g for 30 min
Transfer the supernatant to a new tube
Add 1/10 vol of BN sample buffer
Mix gently
Load 5.5 ul onto BN-gel
Protein standard
|
|
Apoferritin |
β-amylase |
|
5 mg/ml protein stock |
7.5 ul each |
10.0
ul (amylase) |
|
Digitonin Solubilization
buffer |
15.0 ul |
15.0 ul |
|
BN-sample buffer |
3.0 ul |
3.0 ul |
Protein stocks in 20% glycerol, 25 mM BisTrsi-HCl, pH7.0
Mix gently
Load 5.5 ul
|
Protein marker |
Mr (kDa) |
|
Ferritin |
880, 440 |
|
β-amylase |
200 |
|
BSA |
132, 66 |
|
β-lactoglobulin |
35 |
Thyroglobulin (670kD) migrates at position close to ferritin dimer (880kD).
Electrophoresis
We use a Mighty Small Hoefer
setup with a cooling core.
Set a BN gel in a unit connected to a cooling circulator (2-4 C°C in the
cathode tank)
Load samples
Run at constant voltage of 100-200 V, 3-6 hrs.
For immunoblotting or fluorography:
Exchange the cathode buffer (+dye) to cathode buffer lacking the dye after top 1/2 ~2/3 of the gel is covered with dye; then run until the free dye has run off of the bottom of the gel (~2 hrs). The gel should look like this:
For convenience, I put the power supply on a timer when I change to dye-minus cathode buffer. The power supply turns off at the end of the run, but the cooling circulator remains on and the gel stays cold until the next morning, when it can be further processed.
Immunoblotting
Transfer buffer
25 mM Tris, 192 mM Glycine, 20%
Methanol
Use room temperature transfer buffer
to kill peroxidase-like activities.
Incubate BN-gel in 0.1% SDS,
Transfer buffer for ~10 min at RT
0.5 ml 10% SDS + 50 ml Transfer
buffer
Assemble blotting sandwich with PVDF membrane
PVDF membrane must be wet in
methanol before equilibration in transfer buffer
Set in a blotter and run at constant voltage of 50 V for 45 min. - no ice in
the chamber.
Stain the blot with 0.1% PonceauS, 5% acetic acid
It’s a little hard to see marker
proteins.
Destain with 20% MeOH, 7% acetic acid overnight to improve antibody binding. (I've
been skipping any staining and destaining steps; KC.)
Treat the blot like ordinary immunoblotting
Fluorography
Treat with DMSO and then
PPO/DMSO like an SDS-gel.
(It's a little hard to see the MW stds of gels treated this way; I can see the
orange ferritin bands and BSA monomer. Hiroki stains and detains his gels
before PPO/DMSO to see the markers. I don't stain in order to avoid color
quenching; KC)
2-Dimensional Analysis
The BN-gel is run as described above on a 0.75 mm thick gel. The lane of interest is sliced out with a razor blade and then incubated in SDS sample buffer containing 2.5% mercaptoethanol for 10 min. at room temp. or 25°C. The slice is then placed on top of a 1 mm SDS-PAGE gel. We use a BioRad minigel apparatus for this. The stacking gel is poured with a comb that is mostly flat across but has a tooth on one side for mol. weight markers, etc. We've tried sealing with agarose or acrylamide, but it seems to work fine without any sealant. The 0.75 mm gel slice slides nicely onto the 1 mm stacking gel without a lot of pushing and tearing. We always use fresh gel slices (no freezing). Here is a 2D gel done by Lixin Zhang:
Good luck
Hiroki Mori at 7/12/2000
