Team:SDU-Denmark/protocols

From 2010.igem.org

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Protocols <br>
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= Protocols = <br>
''''' Any deviation from these protocols will be noted in the [[https://2010.igem.org/Team:SDU-Denmark/labnotes Labnotes]]
''''' Any deviation from these protocols will be noted in the [[https://2010.igem.org/Team:SDU-Denmark/labnotes Labnotes]]
<br><br>
<br><br>
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__TOC__
__TOC__
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=== Colony PCR ===
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== Colony PCR ==
<br>
<br>
How to amplify DNA from bacteria colonies and solutions <br><br>
How to amplify DNA from bacteria colonies and solutions <br><br>
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[[Image:Team-SDU-Denmark-PCR_protocol.JPG]]
[[Image:Team-SDU-Denmark-PCR_protocol.JPG]]
<br>
<br>
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=== Making competent cells of E. coli for transformation ===
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== Making competent cells of E. coli for transformation ==
<br>
<br>
How to make competent cells for transformation <br><br>
How to make competent cells for transformation <br><br>
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9. Leave the cells on ice for 30 min => now the cells are ready for transformation. <br><br>
9. Leave the cells on ice for 30 min => now the cells are ready for transformation. <br><br>
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=== Transformation ===
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== Transformation ==
<br>
<br>
How to transform compotent cells  
How to transform compotent cells  
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10. Resuspend cells and plate out on LA plates with appropriate antibiotics. <br><br>
10. Resuspend cells and plate out on LA plates with appropriate antibiotics. <br><br>
11. Incubate all plates ON at 37°C <br><br>
11. Incubate all plates ON at 37°C <br><br>
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=== Restriction digest ===
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== Restriction digest ==
<br>
<br>
How to digest DNA using fast digest restriction enzymes. <br><br>
How to digest DNA using fast digest restriction enzymes. <br><br>
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4. Immidiately load the restriction mixture in the gel <br><br>
4. Immidiately load the restriction mixture in the gel <br><br>
5. Run the gel and perform a purification step <br><br>
5. Run the gel and perform a purification step <br><br>
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=== Ligation ===
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== Ligation ==
<br>
<br>
How to assemble DNA biobricks <br><br>
How to assemble DNA biobricks <br><br>
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2. Leave the mixture over-night at 17°C <br><br>
2. Leave the mixture over-night at 17°C <br><br>
3. Test ligation using TAQ-PCR and run test gel afterwards in order to check that the PCR product has the right size <br><br>
3. Test ligation using TAQ-PCR and run test gel afterwards in order to check that the PCR product has the right size <br><br>
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=== DNA extraction from gel (fermentas) ===
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== DNA extraction from gel (fermentas) ==
<br>
<br>
How to extract and purify DNA from gel <br><br>
How to extract and purify DNA from gel <br><br>
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9. Transfer the column into a clean 1.5 mL microcentrifuge tube. Add 50 µL of Elution buffer to the center of the column membrane. Centrifuge for 1 min. <br><br>
9. Transfer the column into a clean 1.5 mL microcentrifuge tube. Add 50 µL of Elution buffer to the center of the column membrane. Centrifuge for 1 min. <br><br>
10. Discard the column and store the purified DNA at -20°C. <br><br>
10. Discard the column and store the purified DNA at -20°C. <br><br>
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=== Genomic DNA purification ===
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== Genomic DNA purification ==
<br>
<br>
How to extract and purify genomic DNA <br><br>
How to extract and purify genomic DNA <br><br>
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7. Measure DNA concentration on nanodrop. <br><br>
7. Measure DNA concentration on nanodrop. <br><br>
8. Store DNA at -20°C <br><br>
8. Store DNA at -20°C <br><br>
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=== Plasmid miniprep kit (Fermentas) ===
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== Plasmid miniprep kit (Fermentas) ==
<br>
<br>
How to isolate plasmids from cultures <br><br>
How to isolate plasmids from cultures <br><br>
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Optional: repeat elution step to increase the overall yield by 10-20%. <br><br>
Optional: repeat elution step to increase the overall yield by 10-20%. <br><br>
11. Discard the column and store the purified plasmid DNA at -20°C. <br><br>
11. Discard the column and store the purified plasmid DNA at -20°C. <br><br>
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=== Preparation of Agarose for gel electrophoresis ===
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== Preparation of Agarose for gel electrophoresis ==
<br>
<br>
How to prepare Agarose for gel electrophoresis.<br><br>
How to prepare Agarose for gel electrophoresis.<br><br>
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5. Cast gel and leave for 20 min until the gel is set. ''Remaining agarose solution is placed in incubater for later use.'' <br><br>
5. Cast gel and leave for 20 min until the gel is set. ''Remaining agarose solution is placed in incubater for later use.'' <br><br>
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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== Preparation of SOB and SOC media ==
<br>
<br>
How to prepare SOB and SOC media for transformation. <br><br>
How to prepare SOB and SOC media for transformation. <br><br>
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1. Cool SOB medium to 60°C <br><br>
1. Cool SOB medium to 60°C <br><br>
2. Add 20mL of 1M glucose. <br><br>
2. Add 20mL of 1M glucose. <br><br>
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=== Making competent cells ===
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== Making competent cells ==
<br>
<br>
How to make competent cells for transformation – the iGem way <br><br>
How to make competent cells for transformation – the iGem way <br><br>
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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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== Measurement of competence ==
<br>
<br>
How to test transformation efficiency of competent cells – the iGEM way <br><br>
How to test transformation efficiency of competent cells – the iGEM way <br><br>

Revision as of 06:56, 13 July 2010