Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(RD1.1)
(Colony PCR)
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1. A single colony is transfered to each eppendorf tube with a pipette tip. (The same tip is used to plate out on a LA+antibiotic plate afterwards) <br>
1. A single colony is transfered to each eppendorf tube with a pipette tip. (The same tip is used to plate out on a LA+antibiotic plate afterwards) <br>
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2. Add 30 ul H2O to each tube.<br>
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2. Add 15 ul H2O to each tube.<br>
3. Microwave with open lid at full power for 2 minutes.<br>
3. Microwave with open lid at full power for 2 minutes.<br>
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4. Prepare Pre-Mix (number of colonies+1) Distribute 17ul to each tube.<br>
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4. Prepare Pre-Mix (number of colonies+1) Distribute 9.5ul to each tube.<br>
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5. Load and set PCR machine<br>
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5. shortly spin down PCR tubes
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6. Add TAQ polymerase at last moment. Make sure to get it under the surface of the solution.<br>
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6. Load and set PCR machine<br>
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7. Run PCR reaction.<br><br>
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7. Add TAQ polymerase at last moment. Make sure to get it under the surface of the solution.<br>
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8. Run PCR reaction.<br><br>
''Pre-mix:''
''Pre-mix:''
<br>
<br>
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5ul 10x TAQ buffer<br>
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2.5ul 10x TAQ buffer<br>
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2ul MgCl2 (Increase in 0.25ul incriments if the DNA you want to extract is longer than 3kb.)<br>
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1ul MgCl2 (Increase in 0.25ul incriments if the DNA you want to extract is longer than 3kb.)<br>
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2ul 10pmol/ul forward primer<br>
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1ul 10pmol/ul forward primer<br>
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2ul 10pmol/ul reverse primer<br>
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1ul 10pmol/ul reverse primer<br>
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1ul 10mM dNTP mix<br>
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0.5ul 10mM dNTP mix<br>
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7ul H2O<br><br>
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3.5ul H2O<br><br>
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1ul TAQ polymerase -> NB! Pre-Mix is made without TAQ polymerase!<br>
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0.5ul TAQ polymerase -> NB! Pre-Mix is made without TAQ polymerase!<br>
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(Try .5ul TAQ polymerase, and adjust H2O, if it works consistentlz this protocol will be updated)
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''PCR program''
''PCR program''
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</table>
</table>
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<br>
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Elongation time is adjusted according to the length of the template. (1 min for every 1Kbp)<br>
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--[[User:Tipi|Tipi]] 07:40, 22 July 2010 (UTC)
== Making competent cells of E. coli for transformation ==
== Making competent cells of E. coli for transformation ==

Revision as of 07:40, 22 July 2010