Revision as of 11:32, 31 October 2017

C O L L A B O R A T I O N S

Calibrations

Collaboration is a powerful driver of progress in science. To stand on the shoulders of giants is increasingly unrealistic in a globalised world where scientists work in ever more specialised areas and without geographic or language barriers.

For science to continue to benefit from globalisation, we must advance the axiom and seek to build a human pyramid from the shoulders before and around us. Collaboration and open source data are at the heart of iGEM and so too the heart of Incell.

Below we describe our most significant collaborations within the iGEM community. The symbiosis we strive for in our project has shone brightly through the partnerships established with teams around the world. Our story — and the stories of our friends — have been mutually shaped by the diversity of our shared experiences, knowledge and perspectives.

**Figure 1** Standard curve of fluorescein fluorescence. Fluorescence in arbitraty units (a.u.), fluorescein concentration in µM.

Introduction

We participated in InterLitab, as we want to be contribute to the scientific progress made through this globe spanning project. In InterLab, 6 test devices are inserted in E.coli D5 α, and the growth and fluorescence is measured.

We used the following plasmids provided by iGEM HQ to transform E.coli:

Positive control
Negative control
Test Device 1: J23101+I13504
Test Device 2: J23106+I13504
Test Device 3: J23117+I13504
Test Device 4: J23101.BCD2.E0040.B0015
Test Device 5: J23106.BCD2.E0040.B0015
Test Device 6: J23117.BCD2.E0040.B0015

Cell measurements

Two colonies from each transformation were picked, and grown in foil-covered 50 ml falcon tubes over night (18 hours).

Preparation OD was measured, and a dilution was calculated to achieve an OD of 0.02. Dilution calculations can be found in the table next to this. Here we used the calculated correction factor from our initial abs/OD calibration. From the absorption measurements taken at 0 hours, we see indications of pipetting errors, as the OD₆₀₀ (average) ranges from 0.015 to 0.6 (table 1).

**Table 1** Starting OD.
	Abs₆₀₀	OD₆₀₀ before	Volume (ml) added to 12 ml media	OD₆₀₀ after dilution (0 hours)
Negative Control (Colony 1)	0,461	1,435	0,167	0,06483974
Negative Control (Colony 2)	0,463	1,439	0,167	0,02584249
Positive Control (Colony 1)	0,450	1,400	0,171	0,04467949
Positive Control (Colony 2)	0,474	1,475	0,163	0,01689103
Test Device 1: J23101+I13504 (Colony 1)	0,462	1,437	0,167	0,03043498
Test Device 1: J23101+I13504 (Colony 2)	0,472	1,469	0,163	0,01977106
Test Device 2: J23106+I13504 (Colony 1)	0,477	1,483	0,162	0,03175824
Test Device 2: J23106+I13504 (Colony 2)	0,454	1,410	0,170	0,018837
Test Device 3: J23117+I13504 (Colony 1)	0,507	1,577	0,152	0,03261447
Test Device 3: J23117+I13504 (Colony 2)	0,492	1,529	0,157	0,01471154
Test Device 4: J23101.BCD2.E0040.B0015 (Colony 1)	0,420	1,307	0,184	0,03759615
Test Device 4: J23101.BCD2.E0040.B0015 (Colony 2)	0,472	1,468	0,163	0,01860348
Test Device 5: J23106.BCD2.E0040.B0015 (Colony 1)	0,513	1,595	0,150	0,04234432
Test Device 5: J23106.BCD2.E0040.B0015 (Colony 2)	0,467	1,451	0,165	0,01494505
Test Device 6: J23117.BCD2.E0040.B0015 (Colony 1)	0,482	1,498	0,160	0,04452381
Test Device 6: J23117.BCD2.E0040.B0015 (Colony 2)	0,455	1,416	0,170	0,02008242

OD₆₀₀

Cell growth stagnated between 4 and 6 hours. Cells transformed with Test Device 1 and 4 grew slower than the 6 other transformations, and even decreased in OD between 4 and 6 hours. Click on figures for enlarged images:

Fluorescence

Some transformed cells continue to increase fluorescence despite a decrease in OD in the same samples. Devices 3 and 6 are very close to the negative control in fluorescence. Click on figures for enlarged images:

Conclusion

Our data indicate which plasmid elements induce the highest production of GFP. Plasmids containing J23117 (Test devices 3 and 6) does not express fluorescence to a higher degree than the negative control. Plasmids with J23101 (Device 1 and 4) induced the highest fluorescence, and plasmids containing J23106 (Test devices 2 and 5) were somewhere in between. Combining the J23101 or J23106 with I13504 (Test devices 1-3) gave a higher fluorescence than adding BCD2.E0040.B0015 (Test devices 4-6).

These results are not reliable on their own, but will be more robust and reliable when combined with data from the other teams participating in the interlab study.

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                      <div class="intro-message2">
 <h3></h3>
-                         <h1>I N T E R  L A B</h1>
+                         <h1>C O L L A B O R A T I O N S</h1>
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-<div class="container">
-            <div>
-                    <div class="clearfix"></div>
-                    <h2 class="section-heading">Introduction </h2>
-                    <p class="lead">We participated in InterLitab, as we want to be contribute to the scientific progress made through this globe spanning project. In InterLab, 6 test devices are inserted in <i>E.coli</i> D5 α, and the growth and fluorescence is measured. <br><br>
-We used the following plasmids provided by iGEM HQ to transform <i>E.coli</i>:
-<ul style="text-align:left; color:white;">
-<li>Positive control</li>
-<li>Negative control</li>
-<li>Test Device 1: J23101+I13504 </li>
-<li>Test Device 2: J23106+I13504 </li>
-<li>Test Device 3: J23117+I13504  </li>
-<li>Test Device 4: J23101.BCD2.E0040.B0015 </li>
-<li>Test Device 5: J23106.BCD2.E0040.B0015 </li>
-<li>Test Device 6: J23117.BCD2.E0040.B0015 </li>
-</ul>
-</p>
-    </div>
-</div>
-</div>
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                  <div class="clearfix"></div>
                      <h2 class="section-heading">Calibrations</h2>
-                     <p class="lead"> Before our measurements began, we performed some calibrations: First an OD<sub>600</sub> reference point for our plate reader, performed with LUDOX according to the protocol. Here we found a correction factor which can be used to calculate OD from measured absorbance. Our correction fator is 3.11. <br><br>
+                     <p class="lead"> Collaboration is a powerful driver of progress in science. To stand on the shoulders of giants is increasingly unrealistic in a globalised world where scientists work in ever more specialised areas and without geographic or language barriers.<br><br>
+For science to continue to benefit from globalisation, we must advance the axiom and seek to build a human pyramid from the shoulders before and around us. Collaboration and open source data are at the heart of iGEM and so too the heart of Incell. <br><br>
+Below we describe our most significant collaborations within the iGEM community. The symbiosis we strive for in our project has shone brightly through the partnerships established with teams around the world. Our story — and the stories of our friends — have been mutually shaped by the diversity of our shared experiences, knowledge and perspectives.
-Secondly we made a fluorescence standard curve with a serial dilution of fluorescein (figure 1). We used the lower 5 data points to calculate a mean µM fluorescein pr a.u. We chose to use the lower concentration range due to two factors: 1) Linearity is better for the lower fluorescein concentrations, and 2) our measured data has a maximum fluorescence of 500, which makes it more important to have a good fit in the lower range.
   </p>
              </div>
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      <!-- /.container -->
 </div>
+<div class="content-section-a">
+<div class="container">
+            <div>
+                    <div class="clearfix"></div>
+                    <h2 class="section-heading">Introduction </h2>
+                    <p class="lead">We participated in InterLitab, as we want to be contribute to the scientific progress made through this globe spanning project. In InterLab, 6 test devices are inserted in <i>E.coli</i> D5 α, and the growth and fluorescence is measured. <br><br>
+We used the following plasmids provided by iGEM HQ to transform <i>E.coli</i>:
+<ul style="text-align:left; color:white;">
+<li>Positive control</li>
+<li>Negative control</li>
+<li>Test Device 1: J23101+I13504 </li>
+<li>Test Device 2: J23106+I13504 </li>
+<li>Test Device 3: J23117+I13504  </li>
+<li>Test Device 4: J23101.BCD2.E0040.B0015 </li>
+<li>Test Device 5: J23106.BCD2.E0040.B0015 </li>
+<li>Test Device 6: J23117.BCD2.E0040.B0015 </li>
+</ul>
+</p>
+    </div>
+</div>
+</div>
 <div class="content-section-a">

Difference between revisions of "Team:UCopenhagen/Collaborations"

Revision as of 11:32, 31 October 2017

C O L L A B O R A T I O N S

Calibrations

Introduction

Cell measurements

OD₆₀₀

Cell growth stagnated between 4 and 6 hours. Cells transformed with Test Device 1 and 4 grew slower than the 6 other transformations, and even decreased in OD between 4 and 6 hours. Click on figures for enlarged images:

Fluorescence

Conclusion

Find Incell here:

Difference between revisions of "Team:UCopenhagen/Collaborations"

Revision as of 11:32, 31 October 2017

C O L L A B O R A T I O N S

Calibrations

Introduction

Cell measurements

OD600 Cell growth stagnated between 4 and 6 hours. Cells transformed with Test Device 1 and 4 grew slower than the 6 other transformations, and even decreased in OD between 4 and 6 hours. Click on figures for enlarged images: ​

Fluorescence

Conclusion

Find Incell here:

OD₆₀₀

Cell growth stagnated between 4 and 6 hours. Cells transformed with Test Device 1 and 4 grew slower than the 6 other transformations, and even decreased in OD between 4 and 6 hours. Click on figures for enlarged images: