Team:SDU-Denmark/protocols

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(Difference between revisions)
(Measurement of competence)
(Making competent cells of E. coli for transformation)
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10. Store at -80°C indefinitely.<br><br>
10. Store at -80°C indefinitely.<br><br>
11. '''Optional:''' Test competence.<br><br>
11. '''Optional:''' Test competence.<br><br>
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=== Measurement of competence ===
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<br>
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How to test transformation efficiency of competent cells – the iGEM way <br><br>
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''Materials''
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<br>
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• pUC19 plasmid (Invitrogen)<br><br>
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• SOC medium (see separate protocol)<br><br>
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''Protocol''
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<br>
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1. Transform 50 µL of competent cells with 1 µL of standard pUC19 plasmid. This is at 10 pg/µL or 10-5 µg/µL (This can be done by diluting 1 µL of NEB pUC19 plasmid (1 µg/µL, NEB part number NS3401S) into 100 mL of TE))<br><br>
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2. Keep on ice for 30 min. <br><br>
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3. Heat shock 60 s. at 42°C '''(Very important)''' <br><br>
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4. Add 250 µL SOC medium <br><br>
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5. Incubate at 37°C for 1 h. in 2 mL centrifuge tubes. (these tubes works well with transformation)<br>
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- Transformation with plasmids pSB1AC3 and pSB1AT3, which are chloramphenicol and tetracycline resistant, incubating for 2 h. yields many more colonies. <br><br>
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6. Plate 20 µL on AMP plates and spread. <br><br>
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7. Incabate plates at 37°C over night. <br><br>
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8. Count the colonies (good cells should yield around 100-400 colonies)
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Transformation efficiency is (dilution factor = 15) x colony x 105/µg DNA <br><br>
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We expect that the transformation efficiency should be between 5x108 and 5x109 cfu/µgDNA <br>
== Transformation ==
== Transformation ==

Revision as of 09:48, 13 July 2010