Team:Grenoble-EMSE-LSU/Documentation/Notebook/May
From 2013.igem.org
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<h1>May</h1> | <h1>May</h1> | ||
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<h2>Week 4 (20-24)</h2> | <h2>Week 4 (20-24)</h2> | ||
<h3>Monday</h3><br><br> | <h3>Monday</h3><br><br> | ||
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<p>We spend some time discovering the equipment at our disposal, how it works and what it can and can't do. We have access to a microplate reader (absorbance and fluorescence), a spectrophotometer (absorbance), an inverted fluorescence microscope, a PCR machine an, multiple centrifuges and electrophoresis machines, and plenty of pipetmans, plastic disposables and gloves. I'm sure there's a couple of things I've forgotten on the list, but at least we know we have what's necessary to start on great footing.<br><br> | <p>We spend some time discovering the equipment at our disposal, how it works and what it can and can't do. We have access to a microplate reader (absorbance and fluorescence), a spectrophotometer (absorbance), an inverted fluorescence microscope, a PCR machine an, multiple centrifuges and electrophoresis machines, and plenty of pipetmans, plastic disposables and gloves. I'm sure there's a couple of things I've forgotten on the list, but at least we know we have what's necessary to start on great footing.<br><br> | ||
- | We have transformed fresh cells with a GFP gene controlled by a PBad promoter using < | + | We have transformed fresh cells with a GFP gene controlled by a PBad promoter using <a href="https://static.igem.org/mediawiki/2013/f/fe/Grenoble_Protocols-TSS_Transformations.pdf"> the TSS method</a></p> |
<h3>Wednesday</h3><br><br> | <h3>Wednesday</h3><br><br> | ||
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<h3>Wednesday</h3> | <h3>Wednesday</h3> | ||
- | <br><br><p>In order to obtain better results in terms of fluorescence and in terms of bacterial growth control, we choose to use M9 for a second experiment to characterize PBAD.<br><br> | + | <br><br><p>In order to obtain better results in terms of fluorescence and in terms of bacterial growth control, we choose to use <a href="https://static.igem.org/mediawiki/2013/5/50/Grenoble_Preparation_of_M9_medium.pdf">M9</a> for a second experiment to characterize PBAD.<br><br> |
M9 is supplemented in glucose. We use <em>E. coli</em> BW25113 which is a prototroph.<br><br> | M9 is supplemented in glucose. We use <em>E. coli</em> BW25113 which is a prototroph.<br><br> | ||
The protocol used is available on the internet. The experiment failed for multiple reasons including lack of controls, lack of time to do every step every 30 minutes. | The protocol used is available on the internet. The experiment failed for multiple reasons including lack of controls, lack of time to do every step every 30 minutes. |
Latest revision as of 01:00, 5 October 2013