Team:Queens Canada/Notebook/Protocols/Rehydration
From 2011.igem.org
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<h3red> Rehydration- Primers</h3red> | <h3red> Rehydration- Primers</h3red> | ||
+ | |||
+ | <regulartext> <b> Storage and Labelling </b> </regulartext> <br> | ||
+ | <regulartext> - Use 2μL of the DNA solution to transform bacteria (in order to amplify the part). Save the remainder of the aqueous DNA in the -20°C freezer. </regulartext> <br> | ||
+ | <regulartext> - Product should be labelled as "DNA (AQ)," using the standard labeling technique, as outlined in the front of your lab book and on the Google Doc. </regulartext> <p> | ||
+ | <regulartext> <b> Materials </b> </regulartext> <br> | ||
+ | <regulartext> - Kit plate, from parts distribution </regulartext> <br> | ||
+ | <regulartext> - ddH2O </regulartext> <p> | ||
+ | <regulartext> <b> Procedure </b> </regulartext> <br> | ||
+ | <regulartext> 1. Ensure that you know the correct year, plate and well for your part. TRIPLE CHECK THIS. Wells are numbered and lettered as shown to the right. <br> | ||
+ | 2. Using sterile technique, load 10μL of diH2O into a p20 pipette.<br> | ||
+ | 3. Pierce the foil of the correct well on the distribution plate, firmly but carefully lower the pipette tip into the very bottom of the well.<br> | ||
+ | 4. Mix the DNA with the water by slowly pumping the water in and out of the pipette tip. You should see the water turn blue if you've done this correctly.<br> | ||
+ | 5. Leaving all of the water in the well, stretch parafilm over the plate and then replace its cover. <br> | ||
+ | 6. Write, "DO NOT TOUCH, KEEP LEVEL" on a piece of tape and affix the tape to the lid of the plate.<br> | ||
+ | 7. Ensuring that you keep the plate level, put it into a 4°C fridge, and leave it there for one hour to allow all of the DNA to dissolve.<br> | ||
+ | 8. Transfer the entire DNA solution from the well into an eppendorf tube.<br> | ||
+ | </regulartext> | ||
</div> | </div> |
Revision as of 12:46, 19 September 2011
5. Briefly vortex again.
6. Aliquot out the correct volume of the concentrated (100 or 200μM) primer solution into an eppendorf tube and dilute it to 100μL solution at the concentration of 10μM (if your concentrated primer solution is 100μM, use 10μL or the concentrated primer and 90μL of water to make your 10μM primer solution).
2. Using sterile technique, load 10μL of diH2O into a p20 pipette.
3. Pierce the foil of the correct well on the distribution plate, firmly but carefully lower the pipette tip into the very bottom of the well.
4. Mix the DNA with the water by slowly pumping the water in and out of the pipette tip. You should see the water turn blue if you've done this correctly.
5. Leaving all of the water in the well, stretch parafilm over the plate and then replace its cover.
6. Write, "DO NOT TOUCH, KEEP LEVEL" on a piece of tape and affix the tape to the lid of the plate.
7. Ensuring that you keep the plate level, put it into a 4°C fridge, and leave it there for one hour to allow all of the DNA to dissolve.
8. Transfer the entire DNA solution from the well into an eppendorf tube.