Difference between revisions of "Part:BBa K3805138:Experience"
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how you used this part and how it worked out. | how you used this part and how it worked out. | ||
| − | == | + | ==Experiments of BBa_K3805138== |
For the synthesis of AIP by agrB-D, we also carried out the corresponding experiments | For the synthesis of AIP by agrB-D, we also carried out the corresponding experiments | ||
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After collecting the standard experimental data, we filtered the 12h culture of the deceiver and mixed the remaining culture with an equal amount of the guard's bacterial solution. 200ul of the culture was placed in a 96-well plate and the mcherry was measured under the ELISA. | After collecting the standard experimental data, we filtered the 12h culture of the deceiver and mixed the remaining culture with an equal amount of the guard's bacterial solution. 200ul of the culture was placed in a 96-well plate and the mcherry was measured under the ELISA. | ||
| − | + | ==result== | |
| − | ==experiment1== | + | ===experiment1=== |
When a certain amount of exogenous AIP was applied to the bacterial fluid, red fluorescence(mCherry) was observed under the microscope. After a period of time, red fluorescence disappeared, and green fluorescence was observed under the microscope. | When a certain amount of exogenous AIP was applied to the bacterial fluid, red fluorescence(mCherry) was observed under the microscope. After a period of time, red fluorescence disappeared, and green fluorescence was observed under the microscope. | ||
| − | ==experiment2== | + | ===experiment2=== |
After a period of testing, we finally got our experimental results | After a period of testing, we finally got our experimental results | ||
Revision as of 15:24, 20 October 2021
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how you used this part and how it worked out.
Experiments of BBa_K3805138
For the synthesis of AIP by agrB-D, we also carried out the corresponding experiments
Experiment1:Toggle Switch Verification
To verify the Bi-stable Switch, we replaced our aimed protein gene with GFP sequence. When a certain amount of exogenous AIP was applied to the bacterial fluid, red fluorescence(mCherry) was observed under the microscope. We then applied a concentration gradient of synthetic AIP to the bacterial fluid to establish an accurate coordination between AIP concentration and mCherry secretion and plotted the corresponding curve.
Experiment 2: Measurement of AIP generation
stage1:Measurement of standard experimental data
We incubated the guards overnight for 12-16h, and then split the experimental material in the ultra-clean bench: five wells of a 96-well plate were poured with 200ul of bacterial solution, followed by 1mM of AIP, and 1ul each of diluted 107, 108 and 109 AIP into the first four wells, leaving a control of the original bacterial solution without AIP.
Then we put the partitioned experimental material into the enzyme marker to detect the fluorescence intensity of mcherry and record the experimental data
stage 2: Deceiver data collection
After collecting the standard experimental data, we filtered the 12h culture of the deceiver and mixed the remaining culture with an equal amount of the guard's bacterial solution. 200ul of the culture was placed in a 96-well plate and the mcherry was measured under the ELISA.
result
experiment1
When a certain amount of exogenous AIP was applied to the bacterial fluid, red fluorescence(mCherry) was observed under the microscope. After a period of time, red fluorescence disappeared, and green fluorescence was observed under the microscope.
experiment2
After a period of testing, we finally got our experimental results
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