Normal SDS-PAGE using Tris-Glycine Gels and Electrophoresis Buffer

From 2010.igem.org

(Difference between revisions)
(New page: '''Wear gloves at all times!''' Requirements: *30% acrylamide(Biorad) '''NEUROTOXIN!''' *4X separation gel buffer: 1.5M Tris.HCl, 0.4% SDS pH6.8 *4X stacking gel buffer: 0.5M Tris.HCl, 1...)
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*10% APS (Ammonium persulfate) ; prepare 10 ml and keep cold in fridge
*10% APS (Ammonium persulfate) ; prepare 10 ml and keep cold in fridge
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Hoeffer Mighty gel system
+
'''Hoeffer Mighty gel system'''
 +
Casting of the gel:
 +
*Per gel take one small glass plate with 'ears', one big white ceramic plate, two grey spacers with perpendicular plastic bits (0.75 mm), and one white comb (0.75 mm)
 +
*Clean the plates etc with soap, rinse with demiwater and ethanol, and dry
 +
*Assemble the system in the gel casting holder. Mark the line of separation/stacking
 +
*Mix the separation gel in 10 ml plastic tube:
 +
                              '''for 2 gels'''
 +
'''Seperation gel (0.75 mm)'''              ''' 12.5%'''            '''16%'''   
 +
    30% acrylamide                      4 ml            5.1 ml
 +
    4X separation buffer                2.4 ml          2.4 ml
 +
    MQ                                  3.2 ml          2.1 ml
 +
    10% APS                            28 μl            28 μl
 +
    TEMED                              28 μl            28 μl
 +
*Pipet the separation gel mix immediately in between the glass plates until the marked line is reached
 +
*Pipet water-saturated isobutanol on top of the polymerizing separation gel
 +
*Let the separation gel polymerize completely before preparing the stacking gel
 +
*When the gel is polymerized, discard the isobutanol and wash the gel with water
 +
*Mix the stacking gel in a 10 ml tube:
 +
                                '''for 2 gels'''
 +
    mQ                              1.92 ml
 +
    4X stacking buffer              0.83 ml
 +
    30% acrylamide                  560 μl
 +
    10% APS                          14 μl
 +
    TEMED                            7 μl
 +
*Pipet the stacking gel mix immediately on top of the separation gel and place the comb without air bubbles. Mark the teeth of the comb with a marker
 +
*Let the gel polymerize (5-30 min); check also the remaining gelmix in the tube
 +
*Disassemble the gel casting holder and take out the gel/plates
 +
*Use the gel immediately or seal the gel in plastic seal bags and store at 4 °C
 +
 
 +
'''Assembly of the Tris-Glycine gel in the electrophoresis unit'''

Revision as of 13:48, 24 August 2010

Wear gloves at all times!

Requirements:

  • 30% acrylamide(Biorad) NEUROTOXIN!
  • 4X separation gel buffer: 1.5M Tris.HCl, 0.4% SDS pH6.8
  • 4X stacking gel buffer: 0.5M Tris.HCl, 1.92M glycine, 1% SDS water saturated isobutanol
  • TEMED( in yellow cabinet )
  • 10% APS (Ammonium persulfate) ; prepare 10 ml and keep cold in fridge

Hoeffer Mighty gel system Casting of the gel:

  • Per gel take one small glass plate with 'ears', one big white ceramic plate, two grey spacers with perpendicular plastic bits (0.75 mm), and one white comb (0.75 mm)
  • Clean the plates etc with soap, rinse with demiwater and ethanol, and dry
  • Assemble the system in the gel casting holder. Mark the line of separation/stacking
  • Mix the separation gel in 10 ml plastic tube: 
                              for 2 gels
Seperation gel (0.75 mm)               12.5%            16%    
   30% acrylamide                      4 ml             5.1 ml
   4X separation buffer                2.4 ml           2.4 ml
   MQ                                  3.2 ml           2.1 ml
   10% APS                             28 μl            28 μl
   TEMED                               28 μl            28 μl
  • Pipet the separation gel mix immediately in between the glass plates until the marked line is reached
  • Pipet water-saturated isobutanol on top of the polymerizing separation gel
  • Let the separation gel polymerize completely before preparing the stacking gel
  • When the gel is polymerized, discard the isobutanol and wash the gel with water
  • Mix the stacking gel in a 10 ml tube: 
                               for 2 gels
   mQ                               1.92 ml
   4X stacking buffer               0.83 ml
   30% acrylamide                   560 μl
   10% APS                          14 μl
   TEMED                            7 μl
  • Pipet the stacking gel mix immediately on top of the separation gel and place the comb without air bubbles. Mark the teeth of the comb with a marker
  • Let the gel polymerize (5-30 min); check also the remaining gelmix in the tube
  • Disassemble the gel casting holder and take out the gel/plates
  • Use the gel immediately or seal the gel in plastic seal bags and store at 4 °C

Assembly of the Tris-Glycine gel in the electrophoresis unit

Retrieved from "http://2010.igem.org/Normal_SDS-PAGE_using_Tris-Glycine_Gels_and_Electrophoresis_Buffer"