Protocol Online: Cached

This is a cached page for the URL (http://wolfson.huji.ac.il/purification/Protocols/Page_SDS.html). To see the most recent version of this page, please click here.

Protocol Online is not affiliated with the authors of this page nor responsible for its content. About Cache

PAGE-SDS Laemmli Protocol

The Protein Purification Facility
The Wolfson Centre for Applied Structural Biology
The Hebrew University of Jerusalem
Dr. Mario Lebendiker
mariol@mail.ls.huji.ac.il Tel: 972-2-6586920

PAGE-SDS Laemmli Protocol

Stock Solutions

1) 1.5M TrisHCl pH 8.3 + 0.4% SDS (adjust pH before you add the SDS). Keep RT.
2) 30% Acrylamide 0.8% Methylene bis Acrylamide or 40% Acrylamide / Methylene bis Acrylamide (ratio: 37.5:1). Keep 4°C
3) 0.5M TrisHCl pH 6.8+ 0.4% SDS (adjust pH before you add the SDS). Keep RT.
4) 10% Ammonium Persulfate (APS). Keep 4°C less than 1 month.

Running Buffer x5

Trizma	0.125M	15.1gr
Glycine	0.96M	72.0gr
SDS	0.5%	5.0gr
H2O up to		1 liter

Keep at RT

Dissolving (Sample) Buffer x5

Glycerol 5ml

SDS 1gr

ß Mercapto Ethanol
(or 0.25M DTT) 2.56ml

0.5M TrisHCl pH 6.8+ 0.4% SDS
2.13ml

Bromo Phenol Blue

traces

Keep in aliquots of 1ml at -20C

Separating Gel

% Acrylamide	10%	10%	12%	12%	15%
Number of Minigels	5	8	5	8	5
1.5M TrisHCl pH 8.3 + 0.4% SDS	7.0 ml	10.5 ml	7.0 ml	10.5 ml	7.0 ml
30% Acrylamide 0.8% Methylene bis Acrylamide	9.3 ml	13.9 ml	11.3 ml	16.9 ml	13.9 ml
H₂O	12.3 ml	18.4 ml	9.3 ml	13.9 ml	6.3 ml
10% APS	100 ul	150 ul	100 ul	150 ul	100 ul
TEMED	23 ul	35 ul	23 ul	35 ul	23 ul

% Acrylamide	10%	10%	12%	12%	15%
Number of Minigels	5	8	5	8	5
1.5M TrisHCl pH 8.3 + 0.4% SDS	7.0 ml	10.5 ml	7.0 ml	10.5 ml	7.0 ml
40% Acrylamide / Methylene bis Acrylamide (ratio: 37.5:1)	7.2 ml	10.8 ml	8.6 ml	12.9 ml	10.8 ml
H₂O	14.4 ml	21.5 ml	12 ml	17.9 ml	9.4 ml
10% APS	100 ul	150 ul	100 ul	150 ul	100 ul
TEMED	23 ul	35 ul	23 ul	35 ul	23 ul

Add TEMED and APS at the end. Gently swirl the flask to mix, being careful not to generate bubbles. Pipette the solution to a level of 4cm of the top. Add 0.3ml of n-buthanol. A very sharp liquid interface will be visible within 10-20min. Let polymerize the gel for another hour at least. Rinse the surface of the gel with watter before pouring the stacking gel.

Stacking Gel

Number of Minigels 2 5 8
Number of Minigels 2 5 8

0.5M TrisHCl pH 6.8+ 0.4% SDS 2.5 ml 4.0 ml 5.2 ml 0.5M TrisHCl pH 6.8+ 0.4% SDS 2.5 ml 4.0 ml 5.2 ml

30% Acrylamide 0.8% Methylene bis Acrylamide 1.0ml 1.5ml 2.0ml 40% Acrylamide / Methylene bis Acrylamide (ratio: 37.5:1) 0.75 ml 1.1 ml 1.4 ml

H₂O 6.4ml 9.6ml 12.8ml H₂O 6.6 ml 10 ml 13.4ml

10% APS 100 ul 150 ul 200 ul 10% APS 100 ul 150 ul 200 ul

TEMED 10 ul 15 ul 20 ul TEMED 10 ul 15 ul 20 ul

Fill each sandwich with stacking gel solution and insert a comb into each place taking care not to trap any bubbles bellow the teeth. The gel should fully polymerized after 1hour. Cover gel with a nylon wrap. Keep gels no more than 2 weeks at 4°C.

Sample Preparation

Prior to adding the sample buffer, keep samples at 0°C. Add the SDS sample buffer (RT) to the sample (still on ice), and boil at 100°C immediately 3 to 5 min. DO NOT leave the sample in SDS sample buffer without heating; endogenous proteases are very active in SDS sample buffer and can cause severe degradation. Once heated, sample could sit at RT for a short time until loading, or at -20°C for a long time.
For a gel thickness of 0.75mm and 15 wells applied 10-25ug protein of a complex mixture, when staining with Coomasie Blue and 0.5 to 5ug for samples for one or few proteins. If silver stain is used 10 to 100-fold less protein can be used.
Samples can be concentrated or interferences (salts, etc.) eliminated with TCA, acetone, TCA-DOC, ethanol, etc. (see attached Protocol). Potassium ions in particular must be removed since they precipitate the SDS.
Some proteins such as nuclear non-histone proteins and membrane proteins, require the presence of 8M urea in the SDS sample buffer to get complete solubilization.
Some membrane bound proteins undergo aggregation at temperatures above 40-50°C. In this case incubate 30min at 40°C with sample buffer.
A shift in the migration distances of proteins with internal disulfide bridges could be observed by incubating samples in SDS in the presence or absence of reducing agents (mercaptoethanol, DTT, DTE, etc)

Staining Solution

Methanol CP 500ml 50%

Acetic Acid CP 100ml 10%

H₂O 400ml

Coomasie Brilliant Blue R 2.5gr 0.25%

Keep flask on dark at RT

Destaining Solution

Methanol CP 150ml 15%

Acetic Acid CP 100ml 10%

H₂O 750ml

Keep flask on dark at RT

Stain overnight at RT or put gel with staining solution 8 sec in microwave on the high position, and then shake for another 15min at RT. Wash with water 2-3 times and distain by several changes of destaining solution in the presence of a sponge.

HOME

EXPRESSION SYSTEMS

EXTRACTION AND CLARIFICATION

PURIFICATION

CHARACTERIZATION

OTHERS

Dr. Mario Lebendiker The Protein Purification Facility
The Wolfson Centre for Applied Structural Biology, The Hebrew University of Jerusalem
mariol@mail.ls.huji.ac.il Tel: 972-2-6586920

Glycerol	5ml
SDS	1gr
ß Mercapto Ethanol (or 0.25M DTT)	2.56ml
0.5M TrisHCl pH 6.8+ 0.4% SDS	2.13ml
Bromo Phenol Blue	traces

Methanol CP	500ml	50%
Acetic Acid CP	100ml	10%
H₂O	400ml
Coomasie Brilliant Blue R	2.5gr	0.25%