Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(TR1.1)
(TR1.1)
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== Transformation ==
== Transformation ==
=== TR1.1 ===
=== TR1.1 ===
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How to transform compotent cells
 
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<br>
''Important remarks''
''Important remarks''
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<br>
'''Positive control with your uncut vector''' <br><br>
'''Positive control with your uncut vector''' <br><br>
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'''Negative control with no DNA''' <br><br>
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'''Negative control with no inserted DNA''' <br><br>
''Materials''  
''Materials''  
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<br>
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• Freshly made compotent E. coli cells. <br><br>
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• Freshly made compotent ''E. coli'' cells. <br><br>
• LA plates with appropriate antibiotics <br><br>
• LA plates with appropriate antibiotics <br><br>
• LB media <br><br>
• LB media <br><br>
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1. Transfer 5 µl DNA (plasmid or ligation mix) to precooled eppendorf tubes. (Use only 1ul if DNA is taken from distribution plates.) <br><br>
1. Transfer 5 µl DNA (plasmid or ligation mix) to precooled eppendorf tubes. (Use only 1ul if DNA is taken from distribution plates.) <br><br>
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2. Transfer 200 µl of cells with to the tube and mix by pipetting up and down '''(keep the cells on ice at all times)''' <br><br>
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2. Transfer 200 µl of competent ''E. coli'' cells to the tube and mix by pipetting up and down '''(keep the cells on ice at all times)''' <br><br>
3. Leave on ice for 30 min. <br><br>
3. Leave on ice for 30 min. <br><br>
4. Heat shock for 90 sec. at 42°C in a water bath, do not shake tubes. <br><br>
4. Heat shock for 90 sec. at 42°C in a water bath, do not shake tubes. <br><br>

Revision as of 13:58, 23 October 2010