Difference between revisions of "Team:TUDelft/Wetlab/Protocols"
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<li>The PCR product(s) can be checked on gel. In order to do so, cast a gel and prepare the samples according to the <a href="#" target="_blank" class="adpbl">DNA electrophoresis </a>protocol.</li> | <li>The PCR product(s) can be checked on gel. In order to do so, cast a gel and prepare the samples according to the <a href="#" target="_blank" class="adpbl">DNA electrophoresis </a>protocol.</li> | ||
</ol> | </ol> | ||
| − | </div> | + | </div> |
| + | |||
| + | <!-- -----------------------COLONY PCR ---------------------------> | ||
| + | <button class="collapsible cadpbl">Colony PCR</button> | ||
| + | <div class="content"> | ||
| + | <p> | ||
| + | <ol> | ||
| + | <li>Under sterile conditions, pick a colony and dilute it in 10 µL of milli-Q water. <br> | ||
| + | <em>NOTE: After you pick the colony, it cannot be used again. It is therefore recommended to make a 'back-up'-plate where you grow the colonies again. This plate should be incubated overnight at 37 °C. </em></li> | ||
| + | <li>Incubate at 90 °C for 10 min. <br> | ||
| + | <em>NOTE: Instead of separate 'cooking' of the cells before the PCR, this step can be incorporated in the PCR program. The initial denaturation step at 98 °C should then be prolonged to 5 minutes (300 seconds). </em></li> | ||
| + | <li>Prepare the GoTaq master mix for all the samples in a single 1.5 mL tube. <br> | ||
| + | <em>NOTE: mind pipetting errors so prepare at little bit more master mix! </em><br> | ||
| + | For one sample: </li> | ||
| + | <table> | ||
| + | <tr > | ||
| + | <th class="tableheaderadpbl">Component</th> | ||
| + | <th class="tableheaderadpbl">Volume (µL)</th> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>GoTaq 5x buffer</td> | ||
| + | <td>10</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>10 mM dNTPs</td> | ||
| + | <td>1</td> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Primer forward (10µM)</td> | ||
| + | <td>1</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>Primer reverse (10µM)</td> | ||
| + | <td>1</td> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Sterile milli-Q</td> | ||
| + | <td>31.8</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>Gotaq polymerase (5u/µL)</td> | ||
| + | <td>0.2</td> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Total</td> | ||
| + | <td>45</td> | ||
| + | </tr> | ||
| + | </table> | ||
| + | <em>* NOTE: Use GoTaq Buffer Green when it is required to run a verification gel afterwards.</em> | ||
| + | |||
| + | <li>Pipette 45 µL of mix into each PCR tube (one tube per colony). </li> | ||
| + | <li>Centrifuge the colony mixture for 5 minutes at 16,000 x g.</li> | ||
| + | <li>Add 5 µL of supernatant of colony mixture to each PCR tube.</li> | ||
| + | <li>Put the tubes in the PCR machine and apply the following program (it needs to be adjusted for primers annealing temperature and extension time): </li> | ||
| + | |||
| + | <br> | ||
| + | <table> | ||
| + | <tr> | ||
| + | <th class="tableheaderadpbl">Step</th> | ||
| + | <th class="tableheaderadpbl">Time (s)</th> | ||
| + | <th class="tableheaderadpbl">Temperature (°C)</th> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Initial denaturation</td> | ||
| + | <td>150</td> | ||
| + | <td>98</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>Denaturation</td> | ||
| + | <td>60</td> | ||
| + | <td>94</td> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Annealing</td> | ||
| + | <td>60</td> | ||
| + | <td>60 (depending on primers)</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>Extension</td> | ||
| + | <td>60 sec per kb DNA</td> | ||
| + | <td>72</td> | ||
| + | </tr> | ||
| + | <tr class="tableunevenadpbl"> | ||
| + | <td>Final extension</td> | ||
| + | <td>600</td> | ||
| + | <td>72</td> | ||
| + | </tr> | ||
| + | <tr class="tableevenadpbl"> | ||
| + | <td>Hold</td> | ||
| + | <td>∞</td> | ||
| + | <td>4</td> | ||
| + | </tr> | ||
| + | </table> | ||
| + | |||
| + | <li>The PCR product(s) can be checked on gel. In order to do so, cast a gel and prepare the samples according to the <a href="#" target="_blank" class="adpbl">DNA electrophoresis </a>protocol.</li> | ||
| + | </ol> | ||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
</div> | </div> | ||
</div> | </div> | ||
Revision as of 14:37, 15 September 2018
Text to write to introduce the protocols
- Under sterile conditions, pick a colony and dilute it in 10 µL of milli-Q water.
NOTE: After you pick the colony, it cannot be used again. It is therefore recommended to make a 'back-up'-plate where you grow the colonies again. This plate should be incubated overnight at 37 °C. - Incubate at 90 °C for 10 min.
NOTE: Instead of separate 'cooking' of the cells before the PCR, this step can be incorporated in the PCR program. The initial denaturation step at 98 °C should then be prolonged to 5 minutes (300 seconds). - Prepare the GoTaq master mix for all the samples in a single 1.5 mL tube.
NOTE: mind pipetting errors so prepare at little bit more master mix!
For one sample: - Pipette 45 µL of mix into each PCR tube (one tube per colony).
- Centrifuge the colony mixture for 5 minutes at 16,000 x g.
- Add 5 µL of supernatant of colony mixture to each PCR tube.
- Put the tubes in the PCR machine and apply the following program (it needs to be adjusted for primers annealing temperature and extension time):
- The PCR product(s) can be checked on gel. In order to do so, cast a gel and prepare the samples according to the DNA electrophoresis protocol.
| Component | Volume (µL) |
|---|---|
| GoTaq 5x buffer | 10 |
| 10 mM dNTPs | 1 |
| Primer forward (10µM) | 1 |
| Primer reverse (10µM) | 1 |
| Sterile milli-Q | 31.8 |
| Gotaq polymerase (5u/µL) | 0.2 |
| Total | 45 |
| Step | Time (s) | Temperature (°C) |
|---|---|---|
| Initial denaturation | 150 | 98 |
| Denaturation | 60 | 94 |
| Annealing | 60 | 60 (depending on primers) |
| Extension | 60 sec per kb DNA | 72 |
| Final extension | 600 | 72 |
| Hold | ∞ | 4 |
- Under sterile conditions, pick a colony and dilute it in 10 µL of milli-Q water.
NOTE: After you pick the colony, it cannot be used again. It is therefore recommended to make a 'back-up'-plate where you grow the colonies again. This plate should be incubated overnight at 37 °C. - Incubate at 90 °C for 10 min.
NOTE: Instead of separate 'cooking' of the cells before the PCR, this step can be incorporated in the PCR program. The initial denaturation step at 98 °C should then be prolonged to 5 minutes (300 seconds). - Prepare the GoTaq master mix for all the samples in a single 1.5 mL tube.
NOTE: mind pipetting errors so prepare at little bit more master mix!
For one sample: - Pipette 45 µL of mix into each PCR tube (one tube per colony).
- Centrifuge the colony mixture for 5 minutes at 16,000 x g.
- Add 5 µL of supernatant of colony mixture to each PCR tube.
- Put the tubes in the PCR machine and apply the following program (it needs to be adjusted for primers annealing temperature and extension time):
- The PCR product(s) can be checked on gel. In order to do so, cast a gel and prepare the samples according to the DNA electrophoresis protocol.
| Component | Volume (µL) |
|---|---|
| GoTaq 5x buffer | 10 |
| 10 mM dNTPs | 1 |
| Primer forward (10µM) | 1 |
| Primer reverse (10µM) | 1 |
| Sterile milli-Q | 31.8 |
| Gotaq polymerase (5u/µL) | 0.2 |
| Total | 45 |
| Step | Time (s) | Temperature (°C) |
|---|---|---|
| Initial denaturation | 150 | 98 |
| Denaturation | 60 | 94 |
| Annealing | 60 | 60 (depending on primers) |
| Extension | 60 sec per kb DNA | 72 |
| Final extension | 600 | 72 |
| Hold | ∞ | 4 |