Justas2010 (Talk | contribs) |
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<p> Fig. 4 </p> | <p> Fig. 4 </p> | ||
− | <p> | + | <p>Fig. 4 A standard curve of fluorescein generated by measuring the fluorescence of serial dilution stock (uM). Fluorescence is plotted against the fluorescein concentration on a logarithmic scale. |
</p> | </p> | ||
<p>During this calibration part we generated a standard curve of fluorescein. Standard curves (linear and on a logarithmic scale) have a 1:1 slope which ensures us that there were no significant mistakes during this calibration part and the data can be used for cell measurement. This allows us to successfully convert cell based readings to an equivalent fluorescein concentration.</p> | <p>During this calibration part we generated a standard curve of fluorescein. Standard curves (linear and on a logarithmic scale) have a 1:1 slope which ensures us that there were no significant mistakes during this calibration part and the data can be used for cell measurement. This allows us to successfully convert cell based readings to an equivalent fluorescein concentration.</p> | ||
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<h4>CELL MEASUREMENTS</h4> | <h4>CELL MEASUREMENTS</h4> | ||
<p>For cell measurements we used the same settings that we used in our calibration measurements. At first, according to the standard protocol we transformed cells with 8 different plasmids (Tab. 1). We picked 2 colonies from each transformation plates and inoculated in 5-10 mL LB medium + Chloramphenicol. We grew the cells overnight (16-18 hours) at 37 °C and 220 rpm. After that we diluted the cultures to a target Abs600 of 0.02. We took samples from these diluted cultures prior to incubation and after 6 hours of incubation measured Abs600 (Fig. 5) and fluorescence (Fig. 6). </p> | <p>For cell measurements we used the same settings that we used in our calibration measurements. At first, according to the standard protocol we transformed cells with 8 different plasmids (Tab. 1). We picked 2 colonies from each transformation plates and inoculated in 5-10 mL LB medium + Chloramphenicol. We grew the cells overnight (16-18 hours) at 37 °C and 220 rpm. After that we diluted the cultures to a target Abs600 of 0.02. We took samples from these diluted cultures prior to incubation and after 6 hours of incubation measured Abs600 (Fig. 5) and fluorescence (Fig. 6). </p> | ||
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+ | <p></p> | ||
+ | <p> Fig. 5 </p> | ||
+ | <p>Fig. 5 Graph comparing the raw Abs600 prior incubation and at hour 6 for each colony using each control/device</p> | ||
+ | <p></p> | ||
+ | <p> Fig. 6 </p> | ||
+ | <p>Fig. 6 Graph comparing the raw fluorescence prior to incubation and at hour 6 for each colony using each control/device</p> | ||
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+ | <p>Comparing absorbance and fluorescence of cells prior to incubation and after 6 hours we can observe that absorbance as well as fluorescence were more intense after 6 h of incubation as it was expected. | ||
+ | Based on the assumption that one bacterial cell gives rise to one colony, colony forming units per 1 mL of an OD600 = 0.1 culture was calculated by counting the colonies on each plate with fewer than 300 colonies and multiplying the colony count by the Final Dilution Factor on each plate The results are shown in Tab. 3.</p> | ||
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+ | <p>Tab. 3. Colony forming units (CFU) per 1 mL of an OD600 = 0.1culture</p> | ||
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+ | <p>Tab. 3</p> | ||
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+ | <p></p> | ||
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</p> <p></p> <p></p> <p></p> <p></p> | </p> <p></p> <p></p> <p></p> <p></p> | ||
Revision as of 22:33, 16 October 2018
InterLab
Abstract
The goal of this year’s InterLab Study was to identify and minimize the sources of systematic variability in fluorescence measurements by normalizing to absolute cell count or colony-forming units (CFUs) instead of optical density (OD).
Participating in the fifth iGEM InterLab Study was a great opportunity to start this year’s competition as well as acquire some valuable knowledge which we implemented into practice during the project.