The following devices were available used for the experiments:

• Positive control
• Negative control
• Test Device 1: J23101 + I13504
• Test Device 2: J23106 + I13504
• Test Device 3: J23117 + I13504
• Test Device 4: J23101.BCD2.E0040.B0015
• Test Device 5: J23106.BCD2.E0040.B0015
• Test Device 6: J23117.BCD2.E0040.B0015

The samples were transformed into the DH5 α E. coli strain by the following transformation protocol:

1. Thaw cells on ice
2. Add DNA and mix
3. Incubate on ice for 1 h
4. Heat-shock 1 min 4 °C
5. Incubate 4 min on ice
6. Add 850 µl 37 °C Luria-Bertani media (LB media) to cells
7. Incubate 1 h 37 °C 900 rpm
8. Centrifuge 4500 rpm 2 min
9. Remove 850 µl liquid
10. Resuspend cells in remaining liquid
11. Grease cell suspension on plates with cAMP resistance
12. Incubate overnight 37 °C

The cells were applied to plates with a chloramphenicol (cAMP) antibiotic with a concentration of 25 µg/ml and incubated over night at 37 °C.

After 16 - 18 hours of incubation two positive colonies for each transformation were transferred to 5 ml liquid media with a chloramphenicol antibiotic with a concentration of 25 µg/ml. The cells were incubated over night at 37 °C at 220 rpm.

The densities of the cultures were measured at OD600 The Tecan Genios Microplate reader was used for the measurement. The samples were diluted to an OD600 = 0.02 in 12 ml LB media with chloramphenicol concentration of 25 µg/ml. The samples were incubated at 37 °C and 220 rpm. Samples of 500 µl were taken after 0, 2, 4 and 6 hours and stored on ice for further experiments. 100 µl of each sample was given into a 96-well plate as in the following pattern:

For the measurement of the OD600 and the GFP fluorescence the Tecan Genios Microplate reader was used. The measurement of the OD600 transparent 96-well-plates were used and for the measurement of the fluorescence black 96-well-plates were used. The reader was calibrated with the following settings.

For the OD600 settings LUDOX-S40 was used as a single setting point. The LUDOX was provided by the iGEM headquarter and enables to obtain a ratiometric conversion factor for a standard OD600 measurement. Four samples of 100 % LUDOX-S40 were measured and as a comparison four samples of 100 % H2O.

For the measurement of the fluorescence a dilution series of fluorescein in four replicates was measured in a 96-well plate. Each well contained 100 µM. The starting concentration was 50 µM. The samples were diluted to: 25; 12.5; 6.25; 3.12; 1.56; 0.78; 0.39; 0.20; 0.1; 0.049; 0 µM. By the measurement of this defined concentrations a standard curve was created. By comparing the fluorescence of the samples to this standard curve, the concentrations of the samples were determined.

The measurements of the calibrations and the samples were performed under the same conditions with an excitation laser of 485 nm and an emission filter of 530/30.

The following data shown in table 1 was received from the LUDOX-S40 calibration.

The following data shown in table 2 was received for the fluorescein standard.

Measurement of OD600 Time point = 0 h

Discussion