IGEM:Cambridge/2008/Notebook/Turing Pattern Formation/2008/08/08: Difference between revisions

Turing Pattern Formation

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Result from the transformationof yesterday Vector Antibiotic Quantity of cells added number of colonies ECE166 Cm5 200μL 0 : problem!!! ECE166 Cm5 100μL 2 ECE166 Cm5 50μL 1 ECE166 Cm10 100μL 0 : no resistance to Cm10! ECE166 (spin) Cm5 100μL a lot, confluent ECE166 (spin) Cm10 100μL 0 ECE166 (glycerol + spin) Cm5 100μL about 150, very small ECE166 (spin) Cm10 100μL 0 ECE153 Spc50 200μL 21 + a lot of confluent colonies ECE153 Spc50 100μL 7 + confluent (a few) ECE153 Spc50 50μL 4 ECE153 (spin) Spc50 100μL 25 + about 200 (small and almost confluent) No DNA Cm5 100μL 0 No DNA Cm10 100μL 0 No DNA Spc50 100μL about 12, maybe more : problem!!!!!

Result for test of ECE112 transformation

On Cm5 plates, we have some colonies for each strains, on Cm5 + Spc 100 plates, no colonies on each plates. This result seems good, however, we forgot to make a control. Since, we had some colonies on control plates, it is possible that our bacillus are resistant to Cm5, even if they are not transformed. We addded some control colonies.

Control with erythromycin

- Prepare erythromycin, stock 5mg/mL : 0.05g in 10mL of SDW

- Prepare plates : add 20μL of Ery (5mg/mL) into 200mL of agar (final concentration : 0.5μg/mL)

- Do several spots on each plate

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Amylase production screening