TAE: Difference between revisions
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* Acetate (100% acetic acid): 57.1 ml | * Acetate (100% acetic acid): 57.1 ml | ||
* [[EDTA]]: 100 ml 0.5M sodium EDTA | * [[EDTA]]: 100 ml 0.5M sodium EDTA | ||
Add dH | Add dH<sub>2</sub>O up to one litre. | ||
To make 1x TAE from 50X TAE stock, dilute 20ml of stock into 980 ml of deionised water. | To make 1x TAE from 50X TAE stock, dilute 20ml of stock into 980 ml of deionised water. | ||
Revision as of 18:57, 9 July 2009
TAE is a commonly used buffer for making and running DNA agarose gels. It offers a few advantages and disadvantages compared to TBE buffer:
- TAE is significantly cheaper to make
- TAE stocks can be 50X concentrated and therefore take up less space than 10X concentrated TBE stock
- TBE offers a higher resolution and has a higher buffering capacity at greater temperatures induced by relatively higher voltages
- TBE can negatively influence the yield of DNA after recovery from a gel when using glass-based protocols. Yield does not seem to be influenced when using silica-based methods.
- The bromide ion in TBE is a powerful inhibitor of enzyme activity. This can prevent degradation of nucleic acid, but can also interfere with subsequent experiments like cloning DNA into a vector.
Ingredients for one litre 50X stock
Add dH2O up to one litre.
To make 1x TAE from 50X TAE stock, dilute 20ml of stock into 980 ml of deionised water. and
