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| | <div class="hull-content">After a transformation has been run and plates have been streaked and patched, overnight cultures will need to be made: | | <div class="hull-content">After a transformation has been run and plates have been streaked and patched, overnight cultures will need to be made: |
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| | <ul><li>Add 10mL of LB broth (not agar) into as many autoclaved conical flasks as | | <ul><li>Add 10mL of LB broth (not agar) into as many autoclaved conical flasks as |
| | needed</li> | | needed</li> |
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| | </section> | | </section> |
| | <input type="radio" name="droptext" id="acc-close" /> | | <input type="radio" name="droptext" id="acc-close" /> |
| − | <input type="radio" name="droptext" id="acc-close" />
| + | <input type="radio" name="droptext" id="cb7" /> |
| − | <input type="radio" name="droptext" id="cb7" /> | + | |
| | <section class="hull"> | | <section class="hull"> |
| − | <label class="hull-title" for="cb7">Running Agarose Gel</label> | + | <label class="hull-title" for="cb7">Protocol for transformation/ heat shock</label> |
| | <label class="hull-close" for="acc-close"></label> | | <label class="hull-close" for="acc-close"></label> |
| − | <div class="hull-content">After the cells have been miniprepped and the plasmid put through a restriction digest, the agarose gel can be run. | + | <div class="hull-content"> |
| | + | This requires chemically competent cells to be made beforehand. These must be stored at -80 |
| | + | degrees Celsius: |
| | <br> | | <br> |
| − | <ul><li>Make up some agarose. This is done by taking 0.5g of agarose powder and putting it in a | + | <ul><li>First, the competent cells and the plasmid intended for transformation must be thawed on |
| − | 250ml sterile conical flask, with 50ml of TAE buffer, then microwaving it in small pulses (20
| + | ice. Additionally, some 1.5ml Eppendorf tubes should be chilled on ice, along with some |
| − | seconds then swirling it around) until it is dissolved. Don’t overheat it or it will evaporate too
| + | pipette tips.</li> |
| − | much. Make up the evaporated volume to 50ml with distilled water.</li>
| + | <li>100ul of the chemically competent cells are then pipetted (using the chilled pipette tip) into |
| − | <li>Add 1 vial of cybersafe (ask technical services for a tube of it and add all of it)</li> | + | a chilled Eppendorf tube.</li> |
| − | <li>Line the white sides of the tank with the agarose solution, to seal it and prevent leakage. Use | + | <li>5ul of DNA is the pipetted into the tube with a chilled tip. This tube is then stored on ice for |
| − | a p1000 pipette set to 1ml. Let it dry (about 5 mins max)</li>
| + | 30 minutes.</li> |
| − | <li>Then pour all the agarose/sybrsafe solution into the tank and put in the comb. Let it set and | + | <li>The tube is then placed in a water bath at 42 degrees Celsius for precisely 90 seconds. After |
| − | solidify (maximum 30 mins)</li>
| + | 90 seconds is up, the tube is transferred back to ice for 2 minutes.</li> |
| − | <li>When the gel has set, remove the comb from the tank (gently!) and then cover the whole | + | <li>900ul SOC medium is then added into the tube (with a normal pipette tip, doesn’t need to |
| − | tank with TAE buffer, so there’s at least half a centimetre of TAE covering the gel.</li>
| + | be chilled) and then mix very gently by pipetting up and down inside the tube.</li> |
| − | <li>Now, the samples need to be loaded. Load some DNA markers (ask technical services for a | + | <li>The tube is then incubated at 37 degrees Celsius for 45 minutes. The tube should not be |
| − | tube of this and load the whole tube) into well 1( left hand side) and then choose what you | + | shaken at all at this point.</li> |
| − | load into wells 2, 3, and 4 etc. (make sure you note what’s in each lane!)</li>
| + | <li>100ul of the transformation mix is then pipetted into the centre of a plate containing LB agar |
| − | <li>Load all of your digests into the wells 2,3, and 4.</li> | + | and the appropriate antibiotic (for example, for plasmid pSB1C3, Chlorophenicol should be |
| − | <li>Plug into a power supply and put the cover on. Run for 40 mins to an hour at 80v. The amps | + | used, and for pSB1A3, use Ampicillin). Use 1ul of antibiotic for each ml of agar.</li> |
| − | don’t matter.</li>
| + | <li>In sterile conditions (Bunsen burner, gloves cleaned with IMS (ALLOWED TO DRY)), spread |
| − | <li>Once the visible markers have reached the half way point of the tank, turn off the power | + | the bacteria around the plate by keeping the lid as closed as possible and inserting the |
| − | supply and drain the TAE buffer form the tank. Remove the gel with a spatula and place in a
| + | spreader then turning the plate around to spread the cells. Then immediately close and |
| − | UV imaging box. Take an image of the gel under UV light, save it onto a USB stick.</li></ul></div>
| + | store upside down.</li> |
| | + | <li>The remained of the transformation mix is then spun at the highest possible speed for 2 |
| | + | minutes. The resulting pellet is then resuspended in 100ul of the existing medium and plated |
| | + | onto the LB and antibiotic plate.</li> |
| | + | <li>Incubate in a 37-degree Celsius incubator for 16-18 hours.</li> |
| | + | <li>Any colonies that result from this should be plated on a patch plate.</li> |
| | + | <li>This is done by taking a plate of LB agar with the appropriate antibiotic and dividing it up |
| | + | into sections by drawing a grid on the bottom. These sections are numbered and then using |
| | + | a sterile pipette tip, the colonies are gently streaked in each section- 1 colony per section.</li></ul></div> |
| | </section> | | </section> |
| | <input type="radio" name="droptext" id="acc-close" /> | | <input type="radio" name="droptext" id="acc-close" /> |
Experiments & Protocols
