Team:Chiba/Sender experiments/Senders(JW1908) T9002(JW1908)
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[[Image:Chiba_talks_JW1908_30_RS3_02.gif|thumb|left|'''Fig.9''' <br>E.coli strain,senders:JW1908,BBa_T9002:JW1908,30°C,Receiver cells/Sender cells = 100.]] | [[Image:Chiba_talks_JW1908_30_RS3_02.gif|thumb|left|'''Fig.9''' <br>E.coli strain,senders:JW1908,BBa_T9002:JW1908,30°C,Receiver cells/Sender cells = 100.]] | ||
- | + | The final fluorescence intensity of the culture containing BBa_K084008 transformed cells which express LVA-tagged RhlI protein was lower than the culture containing cells which express untagged RhlI protein.It shows that LVA-tagged RhlI protein was degraded by LVA-specific protase.However,fluorescence intensity of both cultures increased at the same time.We thought it was because the AHL concentration was quickly reached the threshold concentration and cells began to express gfp.After 2 hours,fluorescence intensity started to increase. | |
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[[Team:Chiba/Project/Experiments:Sender_Crosstalk|>Back to Sender experiment and result]] | [[Team:Chiba/Project/Experiments:Sender_Crosstalk|>Back to Sender experiment and result]] |
Revision as of 05:47, 30 October 2008
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Results and Discussion
Reaction temparature:37°C,09/12
Sender culture:1000μL,Receiver culture:1000μL
Sender culture:100μL,Receiver culture:1000μL
- Green fluorescence intensity didn't increase in the culture containing BBa_K0840010(plac+CinI+LVA).We thought BBa_K084010 didn't work properly or LuxR gene didn't interact with signal molecules synthesized by BBa_K084010.
- Others responded at the same time(4 hours after induction).Final fluorescence intensity differd.
Reaction temparature:37°C
Sender culture:500μLm,Receiver culture:500μL
Left:
- Response time and final fluorescence intensity showed no significant difference.
We thought AHL concentration was quickly reached the threshold concentration.The fluorescence intensity increased as gfp maturured.
Right:
- No significant difference in fluorescence intensity between the culture containing BBa_K084007(plac+RhlI) gene transformed cells and the culture containing BBa_K084008(plac+RhlI(LVA)) gene transformed cells.We thought that the rate of AHL synthesis by each autoinducer synthase was much faster than the rate of its degradation by protease.
Reaction temparature:30°C
Sender culture:500μL,Receiver culture:500μL
Left:
Right:
- No significant difference in fluorescence intensity between the culture containing BBa_K084007(plac+RhlI) gene transformed cells and the culture containing BBa_K084008(plac+RhlI(LVA)) gene transformed cells.We thought that the rate of AHL synthesis by each autoinducer synthase was much faster than the rate of its degradation by protease.
Sender culture:100μL,Receiver culture:1000μL
- No significant difference in fluorescence intensity between the culture containing BBa_K084007(plac+RhlI) gene transformed cells and the culture containing BBa_K084008(plac+RhlI(LVA)) gene transformed cells.We thought that the rate of AHL synthesis by each autoinducer synthase was much faster than the rate of its degradation by protease.
Sender culture:10μL,Receiver culture:1000μL
The final fluorescence intensity of the culture containing BBa_K084008 transformed cells which express LVA-tagged RhlI protein was lower than the culture containing cells which express untagged RhlI protein.It shows that LVA-tagged RhlI protein was degraded by LVA-specific protase.However,fluorescence intensity of both cultures increased at the same time.We thought it was because the AHL concentration was quickly reached the threshold concentration and cells began to express gfp.After 2 hours,fluorescence intensity started to increase.
>Back to Sender experiment and result