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V07_03
V07_03_1: Newly transformed cells are tested via the trypton-whatman-assay
- Experiment:
The cells are dropped onto M9-medium, that are prepared with a 0.5% trypton solution soaked whatman paper. The used strains are DH10B, DH5alpha, XL1, and BL21, each in four variations (empty vector, 18C-, 18O-, 18M-vector)
- Observations & Results:
On the next day, there was no swimming visible at all. After two more (three in total) days, there was strong swimming for the BL21 strains detectable. ∆tar and DH10B strains showed minimal, DH5alpha and XL1 no swimming
V07_03_2: Test of a variety of attractant solutions for the whatman paper
- Experiment:
The swimming assay was performed with ∆tar strains (with empty vector, 18C, and 18M) on M9 agar. For the whatman paper a variety of solutions was tested: Asp+Met, Asp+Leu, Asp+Leu+Met, Trypton, H20. Each solution was used in two different variations, w/ and w/o fluorescin to detect its diffusion over the agar plate.
- Observations & Results:
On the next day, none of the plates showed any swimming. Also, the fluorescin concentration must have been to low, because no fluorescence was detectable under UV light.
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V07_05
Comparison of several attractans for chemotaxis assays
- Experiment:
Wild-type strains without any transformed plasmids were dropped onto M9 agar plates, to identify those that are sensitive for the used chemoattractants (0.5% trypton solution and 50 mM aspartate solution). The chemoattractant was incoroporated into the Whatman paper, which was put in the middle of the agar plate. Furthermore, the influence of chemotaxis-washing-buffer was tested. The approach from above was done twice, once w/ and once w/o a washing step.
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