Team:UC Chile2/General Protocols

From 2012.igem.org

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<li>Thoroughly mix the 3uL of purified parts DNA with the 9uL of 1.33X Gibson assembly master mix in ice</li>
<li>Thoroughly mix the 3uL of purified parts DNA with the 9uL of 1.33X Gibson assembly master mix in ice</li>
<li>Directly incubate the reaction at 50°C for 1 hour</li>
<li>Directly incubate the reaction at 50°C for 1 hour</li>
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<li>Transform competent cells with 8uL of assembled DNA (that leaves 4uL to check in an agarose gel if the reaction fails)</li>
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<li>[[#E. coli Transformation| Transform]] competent cells with 8uL of assembled DNA (that leaves 4uL to check in an agarose gel if the reaction fails)</li>
</ul>
</ul>
<h3>Checking assembly</h3>
<h3>Checking assembly</h3>
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<li>Miniprep colonies and digest plasmid with EcoRI & PstI restriction enzymes</li>
<li>Miniprep colonies and digest plasmid with EcoRI & PstI restriction enzymes</li>
<li>If checking protocols validate until now, proceed by sequencing to corroborate</li>
<li>If checking protocols validate until now, proceed by sequencing to corroborate</li>
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</ul>
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<div id="E.coli Transformation">
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<h1>E.coli Transformation</h1>
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</div>
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<ul>
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<li>Keep 50uL of competent cells[link to TOP10 competent cells protocol from openwetware] in ice (for no more than 10 minutes until transformation)</li>
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<li>Mix 0.01 to 1 total ng of plasmid with competent cells (depending on size of plasmid and competence of your cells)</li>
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<p>Flick very softly to mix (competent cells are very fragile)</p>
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<li>Leave on ice for 30 minutes</li>
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<li>Heat shock at 42°C for 60 seconds</li>
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<li>Add 250uL of LB media</li>
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<li>Incubate at 37°C in a rotating shaker for 1 hour (Ampicillin) or 2 hours (Chloramphenicol and Kanamycin)</li>
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<li>Plate 50uL of transformed cells to a LB agar petri dish with corresponding antibiotic (30ug/mL Kanamycin or 30ug/mL Chloramphenicol or 100ug/mL Ampicillin)</li>
</ul>
</ul>

Revision as of 05:20, 13 September 2012

Project: Luxilla - Pontificia Universidad Católica de Chile, iGEM 2012