Experiment
Symbiosis confirmation ~co-culture assay~ |
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1. Summary of the experiment |
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To accomplish symbiosis of the Company cells and the Customer cells, we mixed and co-cultured the two cells. Company’s characteristics are 4HSL-dependent survival and 3OSC12HSL production, and Company’s characteristics are the opposite from the Customer’s. (If you want to know about the cells in more detail, please visit the project page. Each cells’ functions are confirmed.) These characteristics establish symbiosis between the two cells. This experimentation was focused on confirmation of the symbiosis and its condition. We constructed the Company cells containing GFP and the Customer cells containing RFP. By using the flow cytometer, the symbiosis and the condition become detectable. |
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Fig. 3-1-2 |
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2. Results |
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Fig. 3-3-2. Growth of the two cells when co-cultured |
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3. Materials and methods |
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3-1 Construction |
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-Strain |
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All the samples were JM2.300 strain |
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-Plasmids |
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A. Ptet-GFP-Ptet-RhlR (pSB6A1), Plux-CmR-LasI (pSB3K3) ...Company (type1) |
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B. Ptet-GFP-Ptet-RhiR (pSB6A1), Prhl-CmR-LasI (pSB3K3) ...Company (type2) |
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C. Ptet-GFP-Ptet-RhiR (pSB6A1), Prhl(RL)-CmR-lasI (pSB3K3) ...Company (type3) |
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D. Ptet-RFP-Ptet-LuxR (pSB6A1), Plux-CmR-RhlI (pSB3K3) ...Customer |
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E. Ptet-GFP-Ptet-RhlR (pSB6A1), PlacIq-CmR (pSB3K3) ...Negative control (company) |
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F. Ptet-RFP-Ptet-LuxR (pSB6A1), PlacIq-CmR (pSB3K3) ...Negative control (customer) |
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3-2 Assay Protocol |
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5. Remove the supernatant. | |
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7. Add the suspension to 3mL of LB medium as listed below. | |
LB contains 50 microg / mL ampicilin, 30 microg / mL kanamycin, and Cm. | |
A 30 microL + D 30 microL | |
B 30 microL + D 30 microL | |
C 30 microL + D 30 microL | |
D 30 microL + E 30 microL | |
A 30 microL + F 30 microL | |
B 30 microL + F 30 microL | |
C 30 microL + F 30 microL | |
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(During that time, measure the optical density every one hour.) | |
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4. Reference |
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