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''This figure shows cells size according to the number of cells counted for samples #2. Pink: negative control; black: positive control; yellow: test device 1; blue: test device 2; green: test device 3.'' | ''This figure shows cells size according to the number of cells counted for samples #2. Pink: negative control; black: positive control; yellow: test device 1; blue: test device 2; green: test device 3.'' | ||
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<p style="font-size:11pt">Figures 1 and 2 show that cell population is homogenous between every sample. Cell size is between 10<sup>2</sup> and 10<sup>3</sup> for each sample, and the number of counted cells is almost the same for every sample.</p> | <p style="font-size:11pt">Figures 1 and 2 show that cell population is homogenous between every sample. Cell size is between 10<sup>2</sup> and 10<sup>3</sup> for each sample, and the number of counted cells is almost the same for every sample.</p> | ||
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''This figure shows GFP fluorescence intensity according to the number of cells counted for samples #2. Pink: negative control; black: positive control; yellow: test device 1; blue: test device 2; green: test device 3.'' | ''This figure shows GFP fluorescence intensity according to the number of cells counted for samples #2. Pink: negative control; black: positive control; yellow: test device 1; blue: test device 2; green: test device 3.'' | ||
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<p style="font-size:11pt">Figure 3 and 4 show that fluorescence intensity is correlated to promoter strength of each device. The fluorescence emission level of device 1 is more important than device 2. Device 2 presents a more important fluorescence emission level than device 3. The positive control show a large range of fluorescence intensity, containing two peaks. This probably means that there might be two subpopulations, expressing GFP at different levels. In other terms, two colonies were probably picked and inoculated instead of one in the liquid medium. Those two subpopulations probably don't have the same number of plasmids inside each cell, which leads to different fluorescence emission intensity. However, positive control fluorescence level is around the same as device 2. As expected, negative control does not show any significant fluorescence emission.</p> | <p style="font-size:11pt">Figure 3 and 4 show that fluorescence intensity is correlated to promoter strength of each device. The fluorescence emission level of device 1 is more important than device 2. Device 2 presents a more important fluorescence emission level than device 3. The positive control show a large range of fluorescence intensity, containing two peaks. This probably means that there might be two subpopulations, expressing GFP at different levels. In other terms, two colonies were probably picked and inoculated instead of one in the liquid medium. Those two subpopulations probably don't have the same number of plasmids inside each cell, which leads to different fluorescence emission intensity. However, positive control fluorescence level is around the same as device 2. As expected, negative control does not show any significant fluorescence emission.</p> | ||
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<p style="font-size:11pt">Detailed data (Table I) show that fluorescence intensity results does not vary between two samples of the same construction, except for the positive control. This observation has to be linked with the fact that the positive control cells population might not be homogeneous.</p> | <p style="font-size:11pt">Detailed data (Table I) show that fluorescence intensity results does not vary between two samples of the same construction, except for the positive control. This observation has to be linked with the fact that the positive control cells population might not be homogeneous.</p> | ||
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=Discussion= | =Discussion= | ||
Revision as of 13:54, 4 October 2016