Team:Queens Canada/Parts/Contributions
From 2011.igem.org
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<regulartext> The PCR-Ligation Method of BioBrick Assembly allows the ligation of two linear BioBrick Parts surrounded by the BioBrick prefix and suffix, hereon referred to as Part A (red) and Part B (blue).They can be permanently ligated to each other using the SpeI cut site of Part A and the XbaI cut site of Part B. This linear ligation product is then PCR amplified using the Left Primer of Part A and the Right Primer of Part B. The PCR product then undergoes gel electrophoresis, and the DNA product corresponding to the right length is extracted and purified for further use. </regulartext><p> | <regulartext> The PCR-Ligation Method of BioBrick Assembly allows the ligation of two linear BioBrick Parts surrounded by the BioBrick prefix and suffix, hereon referred to as Part A (red) and Part B (blue).They can be permanently ligated to each other using the SpeI cut site of Part A and the XbaI cut site of Part B. This linear ligation product is then PCR amplified using the Left Primer of Part A and the Right Primer of Part B. The PCR product then undergoes gel electrophoresis, and the DNA product corresponding to the right length is extracted and purified for further use. </regulartext><p> | ||
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+ | <regulartext> During the ligation process, only one of the digestion enzymes, XbaI and SpeI is removed, and one remains in the ligation mixture. If the correct ligation occurred, a permanent scar will result from the ligation of XbaI sticky end to SpeI sticky end that is no longer recognized by either XbaI or SpeI digestion enzymes. The one enzyme remaining in the solution will serve as a selection mechanism for the correct ligation product, and prevent the re-ligation of digested fragments. The removal of one enzyme is necessary for the procedure. If both enzymes remain in the ligation mixture, undesired ligation can occur in which Part B will be ligated to Part A due to the double sticky ends created. However, if both digestion enzymes are removed, there will no longer be a selection mechanism for the correct ligation product. </regulartext> | ||
<regulartext> | <regulartext> |
Revision as of 02:28, 29 September 2011
2. Perform enzymatic cleanup for one of the digest mixtures using EZ-10 PCR Product Purification kit.
3. Mixing of the clean-up product and other digestion product in a 1:1 ratio to obtain a 10 µl mixture.
4. Use the 10 µl mixture and the Fast Ligase System to ligate the two BioBrick parts together.
5. Use the ligation product from the previous step as the template DNA for PCR amplification. Use the 10 µM solution of left primer of BioBrick part A and the 10 µM solution of right primer of BioBrick part B as primers for the PCR Amplification.
6. Follow the instructions in the KAPA HiFi™ Hotstart Kit to perform the PCR reaction. Only 20 to 25 thermocycles are necessary to amplify the ligation product.
7. Create a 1% agarose gel for electrophoresis of the PCR products.
8. With loading dye, load the entire digestion mixture to the 1% agarose gel. Perform gel electrophoresis at 100V and 400 mA for 60 minutes.
9. Using transilluminator, gel extract the visible DNA product corresponding to the right length of the ligation product.
10. Follow the instructions in the Bio Basics EZ-10 Purification Kit, perform purification of the gel extracted products.
11. This gel extracted product may be used for further assembly and processing.