Difference between revisions of "Team:TU Dresden/Notebook/Protocols/AgaroseGel"
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| − | <h2> | + | <h2>Preparation of 0.7% and 2% agarose gel</h2> |
<p style="line-height:1.8;><b>Wear nitrile gloves when preparing the gel, ethidium bromide is considered toxic. </b></p> | <p style="line-height:1.8;><b>Wear nitrile gloves when preparing the gel, ethidium bromide is considered toxic. </b></p> | ||
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<li style="margin-bottom: 10px;line-height:1.8;">0.89 M Boric acid (M<sub>r</sub> 121.14).</li> | <li style="margin-bottom: 10px;line-height:1.8;">0.89 M Boric acid (M<sub>r</sub> 121.14).</li> | ||
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">0.89 M Tris (M<sub>r</sub> 61.83).</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">0.02 M EDTA pH 8.0 500mM stock solution pH 8.0.</li> |
</ul> | </ul> | ||
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<ol> | <ol> | ||
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Dissolve 0.42 g of agarose (0.7%) or 1.2 g of agarose (2%) in 60 mL of 1 x TBE buffer.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Use TBE for making analytical gels and use TAE buffer if gel is meant for DNA or plasmid extraction.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"> | + | <li style="margin-bottom: 10px;line-height:1.8;">Melt the agarose in the microwave until boiling.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Take out the solution and mix it by shaking the bottle.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Put the solution back into the microwave and let it boil again.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Repeat mixing and boiling until the agarose is completely melted.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Set up an agarose gel box with spacers and a comb.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Take out some solution with a blue pipette tip and put it along the inside of the spacers in the gel box and let it solidify.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Add 2 μL of Ethidium Bromide to the remaining solution and mix by shaking the bottle.</li> |
| − | <li style="margin-bottom: 10px;line-height:1.8;"></li> | + | <li style="margin-bottom: 10px;line-height:1.8;">Pour the rest of the solution into the gel box.</li> |
| + | <li style="margin-bottom: 10px;line-height:1.8;">Let it stand for at least 30 minutes until the gel becomes solid.</li> | ||
| + | <li style="margin-bottom: 10px;line-height:1.8;">Fill the gel box up with 1x TBE (or 1x TAE) buffer so that the gel is just covered.</li> | ||
</ol> | </ol> | ||
Latest revision as of 23:24, 13 September 2015
Preparation of 0.7% and 2% agarose gel
Recipe for 10x TBE buffer:
- 0.89 M Boric acid (Mr 121.14).
- 0.89 M Tris (Mr 61.83).
- 0.02 M EDTA pH 8.0 500mM stock solution pH 8.0.
- Dissolve 0.42 g of agarose (0.7%) or 1.2 g of agarose (2%) in 60 mL of 1 x TBE buffer.
- Use TBE for making analytical gels and use TAE buffer if gel is meant for DNA or plasmid extraction.
- Melt the agarose in the microwave until boiling.
- Take out the solution and mix it by shaking the bottle.
- Put the solution back into the microwave and let it boil again.
- Repeat mixing and boiling until the agarose is completely melted.
- Set up an agarose gel box with spacers and a comb.
- Take out some solution with a blue pipette tip and put it along the inside of the spacers in the gel box and let it solidify.
- Add 2 μL of Ethidium Bromide to the remaining solution and mix by shaking the bottle.
- Pour the rest of the solution into the gel box.
- Let it stand for at least 30 minutes until the gel becomes solid.
- Fill the gel box up with 1x TBE (or 1x TAE) buffer so that the gel is just covered.