Difference between revisions of "Team:Lund/InterLab"

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<header class="interlab-landing">
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  <div class="container">
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    <h1 class="description-landing-texts">InterLab</h1>
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<div class="content-wrapper text-layout">
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  <div class="container">
  
<div class="column full_size judges-will-not-evaluate">
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    <div class="row">
<h3>★  ALERT! </h3>
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      <div class="col-md-10">
<p>This page is used by the judges to evaluate your team for the <a href="https://2018.igem.org/Judging/Medals">medal criterion</a> or <a href="https://2018.igem.org/Judging/Awards"> award listed below</a>. </p>
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        <section>
<p> Delete this box in order to be evaluated for this medal criterion and/or award. See more information at <a href="https://2018.igem.org/Judging/Pages_for_Awards"> Instructions for Pages for awards</a>.</p>
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          <h3 class="section-heading">Introduction</h3>
</div>
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          <p>
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            InterLab is a worldwide laborative collaboration where repeatable and reliable results is of very high importance for comparability. In synthetic biology one of the most important signalling proteins is green fluorescent protein (GFP), which fluoresces when exposed to ultraviolet light. Each participating team expressed GFP under promoters of varying strength and compared their measurements to different calibrations.
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          </p>
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        </section>
  
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        <section>
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          <h3 class="section-heading">Materials and Methods</h3>
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          The three different calibration methods were:
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          <br><br>
  
<div class="clear"></div>
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          <p>1. The absorbance at 600 nm was measured for Ludox CL-X of different known concentrations in a plate reader, and OD600 measurements from a spectrophotometer were used to create a conversion factor between absorbance measured by the plate reader and OD600.</p>
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          <p>2. To obtain a standard curve showing the relationship between Abs600 in the plate reader and actual cell count, absorbance of silica beads of the same size as the E. coli cells were measured at different known concentrations. </p>
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          <p>3. The fluorescence intensity of the salt fluorescein, which has similar excitation and emission spectra as GFP, was used to make a standard curve. This standard curve was then used to convert GFP fluorescence measurements into equivalent concentrations of fluorescein, a value which can be used to compare data between different labs regardless of what equipment they use for their measurements.</p>
  
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          <p>All calibrations were done using flat bottomed black 96-well plates. </p>
  
<div class="column full_size">
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          <p>
<h1>InterLab</h1>
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            <i>E. coli</i> DH5-α was transformed with 8 plasmids, each containing different inserts. The only difference between the inserts was the promoter, and for the positive control also the ribosome binding site (Table 1). For full description of the parts visit this page and search for them as stated in Table 1, column “Biobrick”. The cells were incubated according to iGEM measurements protocol for plate readers. The cell density at 600 nm and fluorescence were measured both before and after the incubation.
<h3>Bronze Medal Criterion #4</h3>
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          </p>
<p><b>Standard Tracks:</b> Participate in the Interlab Measurement Study and/or obtain new, high quality experimental characterization data for an existing BioBrick Part or Device and enter this information on that part's Main Page in the Registry. The part that you are characterizing must NOT be from a 2018 part number range.
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<br><br>
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For teams participating in the <a href="https://2018.igem.org/Measurement/InterLab">InterLab study</a>, all work must be shown on this page.
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</p>
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          <table class="table table-bordered">
</div>
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            <caption>Table 1: All tested devices with promoter, promoter strength and RBS</caption>
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            <thead>
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              <tr>
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                <th>Test device</th>
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                <th>Biobrick</th>
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                <th>Promoter strength (a.u)</th>
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                <th>RBS</th>
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              </tr>
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            </thead>
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            <tbody>
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              <tr>
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                <td>Negative control</td>
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                <td>BBa_R0040</td>
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                <td>Medium</td>
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                <td>-</td>
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              </tr>
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              <tr>
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                <td>Positive control </td>
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                <td>BBa_I20270</td>
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                <td> 256</td>
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                <td>B0032</td>
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              </tr>
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              <tr>
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                <td>1</td>
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                <td>BBa_J364000</td>
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                <td>1791</td>
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                <td>B0034</td>
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              </tr>
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              <tr>
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                <td>2</td>
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                <td>BBa_J364001</td>
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                <td>1185</td>
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                <td>B0034</td>
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              </tr>
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              <tr>
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                <td>3</td>
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                <td>BBa_J364002</td>
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                <td>162</td>
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                <td>B0034</td>
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              </tr>
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              <tr>
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                <td>4</td>
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                <td>BBa_J364007</td>
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                <td>547</td>
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                <td>B0034</td>
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              </tr>
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              <tr>
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                <td>5</td>
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                <td>BBa_J364008</td>
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                <td>1831</td>
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                <td>B0034</td>
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              </tr>
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              <tr>
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                <td>6</td>
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                <td>BBa_J364009</td>
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                <td>396</td>
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                <td>B0034</td>
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              </tr>
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            </tbody>
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          </table>
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        </section>
  
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        <section>
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          <h3 class="section-heading">Results</h3>
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          <p>All the raw data is available <a href="https://static.igem.org/mediawiki/2018/b/bd/T--Lund--Interlab_Lund.xlsx">here</a>.</p>
  
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          <p>
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            The results of calibration 1 gave a conversion factor between OD600 and Abs600 of 2.571.
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            The results for calibration 2 can be seen in <em>fig. 1</em>. A quite linear trend was formed.
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            How the fluorescence intensity of the fluorescein salt depended on concentration is shown in <em>fig. 2</em>. Also here a linear trend showed.
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          </p>
  
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          <p>
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            How the cell fluorescence varied before and after the 6 h incubation is shown in <em>fig. 3</em>. Here it was possible to observe an increase for all but the negative control and the 3rd test device.
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          </p>
  
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          <figure>
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            <img class="img-responsive center-block img-thumbnail" src="https://static.igem.org/mediawiki/2018/a/a5/T--Lund--interlab_particles.png">
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            <figcaption>Figure 1: Calibration for Abs600 with varying amounts of particles of the same size as <em>E. coli</em> cells.</figcaption>
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          </figure>
  
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          <figure>
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            <img class="img-responsive center-block img-thumbnail" src="https://static.igem.org/mediawiki/2018/6/6d/T--Lund--interlab_fluor.png">
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            <figcaption>Figure 2: Measured fluorescence for different concentrations of sodium fluorescein. </figcaption>
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          </figure>
  
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          <figure>
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            <img class="img-responsive center-block img-thumbnail" src="https://static.igem.org/mediawiki/2018/b/b2/T--Lund--interlab_cell_od.png">
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            <figcaption>Figure 3: Differences in OD600  before and after 6 h incubation for the different replicates of cells according to <a href="https://static.igem.org/mediawiki/2018/0/09/2018_InterLab_Plate_Reader_Protocol.pdf">measurement protocol</a>. In each colour of <em>fig. 3</em> and <em>fig. 4</em> from left to right, the test devices from top to bottom in table 1 are represented.</figcaption>
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          </figure>
  
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          <figure>
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            <img class="img-responsive center-block img-thumbnail" src="https://static.igem.org/mediawiki/2018/f/f8/T--Lund--interlab_cell_fluorescence.png">
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            <figcaption>Figure 4: Differences in fluorescence before and after 6h incubation of cells for the different replicates.</figcaption>
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          </figure>
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        </section>
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        <section>
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          <h3 class="section-heading">Discussion</h3>
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          <p>According to the promoter strengths, test device 1, 2 and 5 should fluoresce more than the positive control and test device 3 which are the weakest. 4 and 6 should be somewhere in between. </p>
 +
 +
          <p>According to <em>fig. 4</em>, test device 4 was the highest, 2 and 5 medium, 1, 3 and 6 were lower and the controls were low. Thus, the results were not completely off, but matched the expected outcome to some degree. Possible sources of error might be not perfectly regulated cells when it comes to protein production and growth or that the stated strength of the promoters were not what they were in reality. </p>
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        </section>
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      </div>
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    </div>
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  </div>
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</div>
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{{Lund/footer}}

Latest revision as of 01:14, 18 October 2018

InterLab

Introduction

InterLab is a worldwide laborative collaboration where repeatable and reliable results is of very high importance for comparability. In synthetic biology one of the most important signalling proteins is green fluorescent protein (GFP), which fluoresces when exposed to ultraviolet light. Each participating team expressed GFP under promoters of varying strength and compared their measurements to different calibrations.

Materials and Methods

The three different calibration methods were:

1. The absorbance at 600 nm was measured for Ludox CL-X of different known concentrations in a plate reader, and OD600 measurements from a spectrophotometer were used to create a conversion factor between absorbance measured by the plate reader and OD600.

2. To obtain a standard curve showing the relationship between Abs600 in the plate reader and actual cell count, absorbance of silica beads of the same size as the E. coli cells were measured at different known concentrations.

3. The fluorescence intensity of the salt fluorescein, which has similar excitation and emission spectra as GFP, was used to make a standard curve. This standard curve was then used to convert GFP fluorescence measurements into equivalent concentrations of fluorescein, a value which can be used to compare data between different labs regardless of what equipment they use for their measurements.

All calibrations were done using flat bottomed black 96-well plates.

E. coli DH5-α was transformed with 8 plasmids, each containing different inserts. The only difference between the inserts was the promoter, and for the positive control also the ribosome binding site (Table 1). For full description of the parts visit this page and search for them as stated in Table 1, column “Biobrick”. The cells were incubated according to iGEM measurements protocol for plate readers. The cell density at 600 nm and fluorescence were measured both before and after the incubation.

Table 1: All tested devices with promoter, promoter strength and RBS
Test device Biobrick Promoter strength (a.u) RBS
Negative control BBa_R0040 Medium -
Positive control BBa_I20270  256 B0032
1 BBa_J364000 1791 B0034
2 BBa_J364001 1185 B0034
3 BBa_J364002 162 B0034
4 BBa_J364007 547 B0034
5 BBa_J364008 1831 B0034
6 BBa_J364009 396 B0034

Results

All the raw data is available here.

The results of calibration 1 gave a conversion factor between OD600 and Abs600 of 2.571. The results for calibration 2 can be seen in fig. 1. A quite linear trend was formed. How the fluorescence intensity of the fluorescein salt depended on concentration is shown in fig. 2. Also here a linear trend showed.

How the cell fluorescence varied before and after the 6 h incubation is shown in fig. 3. Here it was possible to observe an increase for all but the negative control and the 3rd test device.

Figure 1: Calibration for Abs600 with varying amounts of particles of the same size as E. coli cells.
Figure 2: Measured fluorescence for different concentrations of sodium fluorescein.
Figure 3: Differences in OD600 before and after 6 h incubation for the different replicates of cells according to measurement protocol. In each colour of fig. 3 and fig. 4 from left to right, the test devices from top to bottom in table 1 are represented.
Figure 4: Differences in fluorescence before and after 6h incubation of cells for the different replicates.

Discussion

According to the promoter strengths, test device 1, 2 and 5 should fluoresce more than the positive control and test device 3 which are the weakest. 4 and 6 should be somewhere in between.

According to fig. 4, test device 4 was the highest, 2 and 5 medium, 1, 3 and 6 were lower and the controls were low. Thus, the results were not completely off, but matched the expected outcome to some degree. Possible sources of error might be not perfectly regulated cells when it comes to protein production and growth or that the stated strength of the promoters were not what they were in reality.

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