Team:British Columbia/Notebook/Week 6

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Team: British Columbia - 2011.igem.org

Brainstorming

Week 1: Jun 5-11

Week 2: Jun 12-18

Week 3: Jun 19-25

Week 4: Jun 26-Jul 2

Week 5: Jul 3-9

Week 6: Jul 10-16

Week 7: Jul 17-23

Week 8: Jul 24-30

Week 9: Jul 31-Aug 6

Week 10: Aug 7-13

Week 11: Aug 14-20

Week 12: Aug 21-27

Week 13: Aug 28-Sep 3

Week 14: Sep 4-10

Week 15: Sep 11-17

Week 16: Sep 18-28

Americas Jamboree!!!

Week 19: Oct 9-15

Leading up to the Finals!

Beta-pinene

All 3 transformation plates (P2SDM1, P2SDM2, P2SDM3) have colonies! Marianne set up overnight cultures, mini-prepped them and sent them for sequencing. Hopefully the SDM worked and the beta-pinene synthase gene no longer has illegal cut sites.

(-)-limonene

SDMs have failed thus far. More troubleshooting: use less pfu as the glycerol content in the enzyme could alter the reaction - prepared 3 samples, each with 0.5uL pfu, 1ul pfu, and 2ul pfu, respectively. Also prepare a sample using 0.5 taq polymerase only. Also increased the annealing temperature and elongation time.

Again, gel verification shows no bands. More troubleshooting: use a different cycling condition.

Again, no bands. Something is amiss...

1,8-cineole

After 5 SDMs, transformations and minipreps, Jacob should now have ECORI-less, SPEI-less, XBAI-less, PSTI-less pg-tps-cin and pgxe-tps-cin. The gel of the restriction digest has the correct number of bands. Sequencing is the next step to confirm this result.

IDI1, HMG2 metabolic genes

Yeast colonies were found for HMG2, p330 and Cin, but not IDI1. The yeast transformed with IDI1 did not grow on a URA- plate. This may be because the nutrient marker was mutated in the plasmid, but this would not affect PCR to amplify the gene out. As a precaution, IDI1 was re-amplified.