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| <p>Cell measurements were done to convert the absorbance of the cell suspensions into the absorbance of a known concentration of beads. Then the Colony-Forming Units (CFU) were determined and allowed to obtain a conversion factor from absorbance to CFU. </p> | | <p>Cell measurements were done to convert the absorbance of the cell suspensions into the absorbance of a known concentration of beads. Then the Colony-Forming Units (CFU) were determined and allowed to obtain a conversion factor from absorbance to CFU. </p> |
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− | <p>The next day, the cultures were diluted to an A<sup>600</sup> of 0.02 then their absorbance at 600 nm and fluorescence (excitation: 410 nm, emission: 520 nm, gain= 75) measured with a 96-well plate reader (BMG LABTECH - POLARstar Omega) at 0 and 6 hours. </p> | + | <figcaption style="padding: 10px;"><b>Figure 4 : </b> The cultures were diluted to an A<sup>600</sup> of 0.02 then their absorbance at 600 nm and fluorescence (excitation: 410 nm, emission: 520 nm, gain= 75) measured at 0 and 6 hours. </p> |
| <p>The results showed an increase in the fluorescence and the absorbance after 6 hours compared to the values at 0 hours, indicating an increase in the number of cells (<b>Figure 5</b>). Devices 1 and 4 showed the highest fluorescence while the device 3 was within the same range than the negative control (<b>Figure 5A</b>). Devices 2, 5 and 6 displayed fluorescence levels similar to the positive control. However, we saw no significant difference in absorbance amongst the cells expressing the different devices and the controls at t = 0 h and t = 6 h (<b>Figure 5B</b>). This observation confirms that the fluorescein level observed were not due to a difference in cell number but rather due to different expression levels of the GFP reporter of the devices.</p> | | <p>The results showed an increase in the fluorescence and the absorbance after 6 hours compared to the values at 0 hours, indicating an increase in the number of cells (<b>Figure 5</b>). Devices 1 and 4 showed the highest fluorescence while the device 3 was within the same range than the negative control (<b>Figure 5A</b>). Devices 2, 5 and 6 displayed fluorescence levels similar to the positive control. However, we saw no significant difference in absorbance amongst the cells expressing the different devices and the controls at t = 0 h and t = 6 h (<b>Figure 5B</b>). This observation confirms that the fluorescein level observed were not due to a difference in cell number but rather due to different expression levels of the GFP reporter of the devices.</p> |
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