USTC/Notebook/Running DNA Gels

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*'''Gel-red''' dye, 10,000x.
*'''Gel-red''' dye, 10,000x.
*DNA Marker DL2000 and DL15000.
*DNA Marker DL2000 and DL15000.
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*Melted '''Agarose''' in 1xTAE.
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*melting appropriate amount of Agarose mixed in TAE in the microwave. (eg. to prepare 100ml of melted 1% agarose, mix 1g of agarose in ~99ml 1xTAE in a foil-covered flask and microwave for 4+min; keep an eye on it every couple of minutes when you microwave so it doesn't boil over; be careful to wear gloves when handling hot liquid containers). Can leave on bench and re-melt every time you need it.
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Preparation
 +
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Make a 1% agarose solution in 100ml TAE, for typical DNA fragments. A solution of up to 2-4% can be used if you analyze small DNA molecules, and for large molecules, a solution as low as 0.7% can be used.
 +
Carefully bring the solution just to the boil to dissolve the agarose, preferably in a microwave oven.
 +
Let the solution cool down to about 60 °C at room temperature, or water bath. Stir or swirl the solution while cooling, Wearing gloves from here on.
 +
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Add 10 µl Gel-Red(10000X) per 100 ml gel solution for a final concentration of 0.5 ug/ml. Be very careful when handling the concentrated stock.
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Stir the solution to disperse the gel-red, then pour it into the gel rack.
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Insert the comb at one side of the gel, about 5-10 mm from the end of the gel.
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When the gel has cooled down and become solid, carefully remove the comb. The holes that remain in the gel are the wells or slots.
 +
Put the gel, together with the rack, into a tank with TAE. Ethidium bromide at the same concentration can be added to the buffer. The gel must be completely covered with TAE, with the slots at the end electrode that will have the negative current.

Revision as of 16:24, 27 October 2008

< Back to Notebook

Running DNA Gels

Materials

  • DNA, the thing you want to analyze/cut out. Measure concentration in nanodrop beforehand.
  • 1xTAE buffer.
  • Gel-red dye, 10,000x.
  • DNA Marker DL2000 and DL15000.
  • Melted Agarose in 1xTAE.
  • melting appropriate amount of Agarose mixed in TAE in the microwave. (eg. to prepare 100ml of melted 1% agarose, mix 1g of agarose in ~99ml 1xTAE in a foil-covered flask and microwave for 4+min; keep an eye on it every couple of minutes when you microwave so it doesn't boil over; be careful to wear gloves when handling hot liquid containers). Can leave on bench and re-melt every time you need it.

Preparation

Make a 1% agarose solution in 100ml TAE, for typical DNA fragments. A solution of up to 2-4% can be used if you analyze small DNA molecules, and for large molecules, a solution as low as 0.7% can be used. Carefully bring the solution just to the boil to dissolve the agarose, preferably in a microwave oven. Let the solution cool down to about 60 °C at room temperature, or water bath. Stir or swirl the solution while cooling, Wearing gloves from here on.

Add 10 µl Gel-Red(10000X) per 100 ml gel solution for a final concentration of 0.5 ug/ml. Be very careful when handling the concentrated stock. Stir the solution to disperse the gel-red, then pour it into the gel rack. Insert the comb at one side of the gel, about 5-10 mm from the end of the gel. When the gel has cooled down and become solid, carefully remove the comb. The holes that remain in the gel are the wells or slots. Put the gel, together with the rack, into a tank with TAE. Ethidium bromide at the same concentration can be added to the buffer. The gel must be completely covered with TAE, with the slots at the end electrode that will have the negative current.