Revision as of 02:07, 12 October 2018

Interlab

Introduce

As one of the most important measurement marker in synthetic biology,however, the fluorescence data of GFP usually cannot be compared because it has been reported in different units or because different groups process data in different ways.

The goal of the iGEM InterLab Study is to identify and correct the sources of systematic variability in synthetic biology measurements, so that eventually, measurements that are taken in different labs will be no more variable than measurements taken within the same lab,

The goal for the fifth interlab is to reduce lab-to-lab variability in fluorescence measurements by normalizing to absolute cell count or colony-forming units (CFUs) instead of OD.

Methods

First, make three sets of unit calibration measurements: an OD600 reference point, a particle standard curve, and a fluorescein standard curve.

Second, perform the cell measurements.

Finally, Fill in the experimental data as required.

Click here to see the complete method.

Results

Standard Curve

Figure 1.2 particle stanard cure — **Figure1.1 OD600 reference point tab**

Measurement

Figure 2.2 Abs600 Raw Reading — **Figure 2.1 Fluorescence Raw Reading**

Fluorescence per colony

**Figure 3.1 Fluorescence per OD at 0h**

Figure 3.2 Fluorescence per OD at 6h — **Figure 3.1 Fluorescence per OD at 0h**

Discussion

Highest average fluorescence was obtained from test device 5, closely followed by device 4 and test device 1.Test device 6 and test device 2 show a modest fluorescence intensity, while test devices 3 have any fluorescence signal as well as the negative group. The order of the promoters given by igem official website is, from strong to weak.test device 4,test device5,test deviece1,test device2,test device6,and test device3. The experimental value is in line with the expected value.

Comparing the fluorescence values at 0h and 6h, it was found that the fluorescence value at 6h did not increase significantly. According to the given protocol from iGEM, the 0h bacterial liquid is not directly measured by fluorescence, but is measured after 6 hours of ice bath. We believe that the ice bath is not conducive to bacterial growth, so a large amount of fluorescent protein is expressed. The experiment confirmed our conjecture. If the 0h bacteria solution is directly measured instead of ice bath, the fluorescence value will be significantly lower than the fluorescence value of 6h.

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