Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(Ligation)
(Preparation of SOB and SOC media)
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6. Load gel and run gel. ''Load only 5 µL of DNA marker'' <br><br>
6. Load gel and run gel. ''Load only 5 µL of DNA marker'' <br><br>
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== Preparation of SOB and SOC media ==
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<br>
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How to prepare SOB and SOC media for transformation. <br><br>
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=== SOB medium ===
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<p style="text-align: justify;">
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<br>
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Used in growing bacteria for preparing chemically compotent cells. <br><br>
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''Materials''
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<br>
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For 1 L:<br>
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• 20 g tryptone <br><br>
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• 5 g yeast extract <br><br>
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• 0.5g NaCl <br><br>
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• dH2O to 1 L <br><br>
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• KCl (is made by dissolving 1.86 g of KCl in 100 mL of deionized H2O)<br><br>
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• 2M MgCl2 (is made by dissolving 19g MgCl2 in 90 mL dH2O =>adjust to obtain a volume of 100 mL using dH2O => autoclavate)<br><br>
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''Protocol''
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<br>
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1. Add tryptone, yeast extract and NaCl to 950 mL of dH2O and shake until solute has dissolved. <br><br>
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2. Add 10 mL of 250 mM solution of KCl <br><br>
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3. Adjust volume to 1 L using dH2O <br><br>
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4. Autoclavate for 20 min. <br><br>
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5. Just before use add 5 mL of sterile solution of 2M MgCl2 <br><br>
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=== SOC medium ===
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<p style="text-align: justify;">
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<br>
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''Materials''
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<br>
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• SOB medium. <br><br>
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• 1M glucose (is made by dissolving 18g of glucose in 90 mL of dH2O => adjust to obtain a volume of 100 mL using dH2O)<br><br>
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''Protocol''
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1. Cool SOB medium to 60°C <br><br>
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2. Add 20mL of 1M glucose. <br><br>
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== Extraction af Carotenoids and polyene chromophores ==
== Extraction af Carotenoids and polyene chromophores ==
=== EX1.1 ===
=== EX1.1 ===

Revision as of 15:27, 23 October 2010