"
Team:Newcastle/Gel electrophoresis
From 2010.igem.org
(Difference between revisions)
Shethharsh08 (Talk | contribs) |
|||
| Line 4: | Line 4: | ||
==Materials== | ==Materials== | ||
| - | # | + | * 50X TAE buffer |
| - | # | + | *# Make up 1 liter of 50X TAE buffer with the following: |
| - | # | + | *# 242g of TRIS base |
| - | # | + | *# 57.1 ml of acetic acid |
| - | # Gel making tank | + | *# 100 ml of 0.5 M of EDTA (pH 8.0) |
| - | + | *# Top up to 1 liter with water | |
| + | * SafeView | ||
| + | * Agarose | ||
| + | * Eppendorf | ||
| + | * Gel making tank | ||
| + | * Gel running tank | ||
==Procedures== | ==Procedures== | ||
Revision as of 10:11, 30 July 2010
| |||||||||||||
| |||||||||||||
Gel electrophoresis
Materials
- 50X TAE buffer
- Make up 1 liter of 50X TAE buffer with the following:
- 242g of TRIS base
- 57.1 ml of acetic acid
- 100 ml of 0.5 M of EDTA (pH 8.0)
- Top up to 1 liter with water
- SafeView
- Agarose
- Eppendorf
- Gel making tank
- Gel running tank
Procedures
- Make up 1% agarose gel (1 g of agarose in 100 ml of TAE buffer) and transfer 60 ml of molten agarose gel into the gel tray with 3 μl of Safeview dye.
- Wait for 30 min to allow the gel to harden.
- Transfer harden gel into the gel tank and add TAE buffer until the gel is completely submerge.
- Depending on the nature of the sample, 3μl of GeneRuler™ 1kb Plus DNA Ladder was used for analysing DNA.
- Loading buffer was then added together with the sample before loading onto the gel matrix.
- Run gel at 90V until separation is achieved and visualize using the gelDoc.
Go back to our Protocol List
   
|
    
|
