Team:ETH Zurich/lab/protocols

From 2014.igem.org

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(Multi site directed mutagenesis)
(Methods)
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==Methods==
==Methods==
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===Preparation of competent ''E. coli''===
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===Preparation of chemically competent ''E. coli''===
   
   
Day before: Preparation of a Top10 cells preculture  in LB-medium containing streptomycin (25 μg/mL)
Day before: Preparation of a Top10 cells preculture  in LB-medium containing streptomycin (25 μg/mL)
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===Preparation of electrocompetent ''E. coli''===
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# Grow a 5mL suspension of your cells of interest to OD=0.6
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# Pre-cool your centrifuge to 4°C
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# Pre-cool autoclaved water on ice
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# Cool the cells on ice for 5-10 minutes
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# Centrifuge for 6 minutes
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# Discard supernatant
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# Resuspend pellet with 1mL of chilled water
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# Centrifuge for 6 min
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# Repeat washing step followed by centrifugation 3 times
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# After last centrifugation step, discard supernatant and resuspend pellet in 50uL chilled water.
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# Electroporate
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# Add SOC medium and let cells recover at 37°C for 1 hour
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# Streak on LB-Agar plates with the corresponding antibiotic
===Preparation of DNA from iGEM kit===
===Preparation of DNA from iGEM kit===
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<html><article id='devices'></html>
<html><article id='devices'></html>
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==Devices==
==Devices==

Revision as of 09:58, 11 October 2014

iGEM ETH Zurich 2014