<p>Our InterLab Study Lab Book can be found <a href"https://2015.igem.org/Team:Aalto-Helsinki/InterLabBook">here</a> for a fully detailed overview of our study.</p>
+
<p>Our InterLab Study Lab Book can be found <a href="https://2015.igem.org/Team:Aalto-Helsinki/InterLabBook">here</a> for a fully detailed overview of our study.</p>
<h2>Devices</h2>
<h2>Devices</h2>
Revision as of 23:56, 8 September 2015
InterLab Study
Our InterLab Study Lab Book can be found here for a fully detailed overview of our study.
Devices
The following devices were created in a backbone pSB1C3: ⚫ J23101 + I13504 (B0034-E0040-B0015) ⚫ J23106 + I13504 (B0034-E0040-B0015). However, constructing a device J23117 + I13504 (B0034-E0040-B0015) wasn't successful due to the time limit and limited ligation times. More details available on Lab Book. The device sizes were analyzed with restriction mapping which results can be seen in Figure 1.Used BBa_I20270, a GFP expressing part in the pSB1C3 backbone as a positive control. Negative controls were organisms with an empty plasmid and without any vector.
Protocols
Constructing devices
Protocols for the restriction, ligation and transformation of BioBricks can be found here.
Cultivations and measurement
Followed the next protocol for preparing the samples:Streaked out LB-plates with E.coli TOP10 strain containing every device and control with chloramphenicol concentration of 35ug/ml. Incubated plates overnight (18-20 hours) at 37C. Picked up biological triplates from the plates and inoculated 3 ml liquid cultures from the colonies with 12ml polypropylene test tube. Incubated the tubes at 37C with shaking at 300rpm for 18 hours. Measured OD600 values of cultures in cuvettes and calculated the dilution required for each sample to obtain the OD value of 0,5. Diluted and re-measured the samples to reach 5% accuracy of 0,5. Transfered 200ul of each sample into 96-well transparent plate and set the platereader to read fluorescence intensity. Proceed with the measurements with the following equipment: Type: Cell Imaging Multi-Mode Plate Reader
Name and model: Cytation 3
Company: BioTek Instruments, Inc
The following parametres were used:
Excitation wavelength: 470 nmEmission wavelength: 511 nmOptics Position: Bottom Filter: Quadruple Monochromators with Bandwith of 16 nm Units Reported: RFU
Results
Most samples generated overflow values which could not be measured with the plate reader. The incubation may have generated too much fluorescence proteins even though the samples were diluted properly. The problem wasn't solved after new dilutions of 9:10 ratio and due to the time limit, other ratios weren't attempted.
1st Technical Replicon
Sample
J23117 + I13504
J23101 + I13504
J23151
Empty backbone
Without backbone
Blanks
1
OVRFLW
83954
53925
16309
13663
29336
2
OVRFLW
OVRFLW
56764
16335
14148
14940
3
OVRFLW
OVRFLW
61918
16771
14073
2nd Technical Replicon
Sample
J23117 + I13504
J23101 + I13504
J23151
Empty backbone
Without backbone
Blanks
1
OVRFLW
85224
53553
16307
13747
29470
2
OVRFLW
OVRFLW
56472
16204
14267
14972
3
OVRFLW
OVRFLW
60969
16818
14381
3rd Technical Replicon
Sample
J23117 + I13504
J23101 + I13504
J23151
Empty backbone
Without backbone
Blanks
1
OVRFLW
86750
56390
16123
13536
30778
2
OVRFLW
OVRFLW
58294
16294
14207
14856
3
OVRFLW
OVRFLW
62229
16793
13994
Restriction Map
The gel electrophoresis mapping of J23101 + I13504 and J23106 + I13504 can be seen in Figure 1.
Figure 1. Restriction mapping for J23101 + I13504 and J23106 + I13504.
Comments are missing because the figure will be changed later . The sizes of samples seems to be slightly bigger than expected so a new restriction and gel run will be proceeded during the week 37. The explanations for ladders and scaling will be updated then.
