Team:Gdansk-UG/Notebook

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<td align="left" valign="top"><table width="815" border="0" cellpadding="0" cellspacing="0" class="topMenu">
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              <tr>
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                <td width="67" height="56" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG">Home</a></td>
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                <td width="109" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Team" title="Our stories">Team</a></td>
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                <td width="104" align="center" valign="middle"><p><a href="https://igem.org/Team.cgi?year=2013">Official</a></p>
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                <p><a href="https://igem.org/Team.cgi?year=2013">Team Profile</a></p></td>
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                <td width="82" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Project">Project</a></td>
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                <td width="116" align="center" valign="middle"><p><a href="https://2013.igem.org/Team:Gdansk-UG/Parts">Parts Submitted</a></p>
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                  <a href="https://2013.igem.org/Team:Gdansk-UG/Parts">                  to the Registry</a></td>
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                <td width="86" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Modeling">Human Practice</a></td>
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                <td width="99" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Notebook">Notebook</a></td>
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                <td width="68" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Safety">Safety</a></td>
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                <td width="82" align="center" valign="middle"><a href="https://2013.igem.org/Team:Gdansk-UG/Attributions">Attributions</a></td>
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              <tr>
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                <td width="760" height="42" align="left" valign="top">&nbsp;</td>
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              <tr>
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                <td height="91" align="left" valign="top"><p>Week 1<br />
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                  6 flasks  were prepared with different alcohol concentration for determining <em>M.organophilum</em> tolerance to methanol,  tolerance of aerobic conditions and tolerance to ethanol. <br />
 +
                  Medium used  for cultivating <em>M.organophilum</em> contains:</p>
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                  <ul>
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                    <li>5g  peptone</li>
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                    <li>3g  meat extract</li>
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                    <li>Distilled  water to 1l</li>
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                    <li>pH  adjusted to 7.0</li>
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                    <li></li>
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                    <li><img src="https://static.igem.org/mediawiki/2013/e/ee/Attributions_clip_image001.png" alt="plik1" width="542" height="287" /></li>
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                    <li></li>
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                    <li></li>
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                  </ul>
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                  <table border="1" cellspacing="0" cellpadding="0" align="left">
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                    <tr>
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                      <td width="28" valign="top"><p>#</p></td>
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                      <td width="324" valign="top"><p>Content of flask</p></td>
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                      <td width="95" valign="top"><p>OD600 after 2 hours</p></td>
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                      <td width="83" valign="top"><p>OD600&nbsp; <br />
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                        25.06.13</p></td>
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                      <td width="82" valign="top"><p>OD600<br />
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                        26.06.13</p></td>
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                      <td width="83" valign="top"><p>OD600<br />
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                        28.06.13.13</p></td>
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                      <td width="80" valign="top"><p>OD600<br />
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                        04.07.13</p></td>
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                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>1</p></td>
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                      <td width="324" valign="top"><p>1% methanol</p></td>
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                      <td width="95" valign="top"><p>0,109</p></td>
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                      <td width="83" valign="top"><p>0,06</p></td>
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                      <td width="82" valign="top"><p>0,138</p></td>
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                      <td width="83" valign="top"><p>0,145</p></td>
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                      <td width="80" valign="top"><p>0,184</p></td>
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                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>2</p></td>
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                      <td width="324" valign="top"><p>1% under layer of    paraffin</p></td>
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                      <td width="95" valign="top"><p>0,06</p></td>
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                      <td width="83" valign="top"><p>0,071</p></td>
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                      <td width="82" valign="top"><p>0,117</p></td>
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                      <td width="83" valign="top"><p>0,155</p></td>
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                      <td width="80" valign="top"><p>0,461</p></td>
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                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>3</p></td>
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                      <td width="324" valign="top"><p>2% methanol</p></td>
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                      <td width="95" valign="top"><p>0,055</p></td>
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                      <td width="83" valign="top"><p>0,066</p></td>
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                      <td width="82" valign="top"><p>0,086</p></td>
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                      <td width="83" valign="top"><p>0,210</p></td>
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                      <td width="80" valign="top"><p>0,450</p></td>
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                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>4</p></td>
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                      <td width="324" valign="top"><p>1% ethanol</p></td>
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                      <td width="95" valign="top"><p>-0,08</p></td>
 +
                      <td width="83" valign="top"><p>0,078</p></td>
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                      <td width="82" valign="top"><p>0,047</p></td>
 +
                      <td width="83" valign="top"><p>0,073</p></td>
 +
                      <td width="80" valign="top"><p>0,071</p></td>
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                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>5</p></td>
 +
                      <td width="324" valign="top"><p>2% ethanol</p></td>
 +
                      <td width="95" valign="top"><p>0,07</p></td>
 +
                      <td width="83" valign="top"><p>-0,013</p></td>
 +
                      <td width="82" valign="top"><p>0,047</p></td>
 +
                      <td width="83" valign="top"><p>0,067</p></td>
 +
                      <td width="80" valign="top"><p>0,079</p></td>
 +
                    </tr>
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                    <tr>
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                      <td width="28" valign="top"><p>6</p></td>
 +
                      <td width="324" valign="top"><p>5% ethanol</p></td>
 +
                      <td width="95" valign="top"><p>0,02</p></td>
 +
                      <td width="83" valign="top"><p>0,076</p></td>
 +
                      <td width="82" valign="top"><p>0,031</p></td>
 +
                      <td width="83" valign="top"><p>0,011</p></td>
 +
                      <td width="80" valign="top"><p>0,033</p></td>
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                    </tr>
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                  </table>
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                  <p><strong></strong></p>
 +
                  <p>Week 2<br />
 +
                    Inoculating  liquid medium with <em>E.coli </em>TOP10 F&rsquo; (in preparation for transformation).<strong></strong><br />
 +
                    OD600&nbsp; of E.coli after one night &ndash; 0,718<br />
 +
                    Preparing competent <em>E.coli</em> TOP10 F&rsquo; cells.<br />
 +
                    Transformation of <em>E.coli</em> with iGEM Transformation  efficiency Kit according to protocol provided by iGEM - <a href="http://parts.igem.org/Help:Transformation_Efficiency_Kit">http://parts.igem.org/Help:Transformation_Efficiency_Kit</a><strong>. </strong> <br />
 +
                    Transformation of <em>E.coli </em>TOP10 F&rsquo; cells with BioBricks:</p>
 +
                  <ul>
 +
                    <li>BBa_K316003  &ndash; 3C in plate 1</li>
 +
                    <li>BBa_K823017  &nbsp;- 3D in plate 1</li>
 +
                    <li>BBa_K895006  &nbsp;- 15L in plate 1</li>
 +
                  </ul>
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                  <p>Incubation in 37&deg; C.<br />
 +
                    Transformation results:</p>
 +
                  <table border="1" cellspacing="0" cellpadding="0">
 +
                    <tr>
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                      <td width="384" valign="top"><br />
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                        Plasmid </td>
 +
                      <td width="384" valign="top"><p>Number of colonies</p></td>
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                    </tr>
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                    <tr>
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                      <td width="384" valign="top"><p>Control (without plasmid)</p></td>
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                      <td width="384" valign="top"><p>0</p></td>
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                    </tr>
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                    <tr>
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                      <td width="384" valign="top"><p>3C</p></td>
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                      <td width="384" valign="top"><p>2</p></td>
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                    </tr>
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                    <tr>
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                      <td width="384" valign="top"><p>3D</p></td>
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                      <td width="384" valign="top"><p>0</p></td>
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                    </tr>
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                    <tr>
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                      <td width="384" valign="top"><p>15L</p></td>
 +
                      <td width="384" valign="top"><p>4</p></td>
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                    </tr>
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                  </table>
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                  <p>Inoculation of plates with basic medium and 25mg/l chloramphenicol with colonies from 3C and 15L  plate. <br />
 +
                    Week 3<br />
 +
                    Inoculation liquid medium with cholamphenicol (25mg/l) with 1 colony of transformed <em>E.coli</em> (3C and 15L).<br />
 +
  <strong>&nbsp;</strong>Inoculating liquid medium with <em>E.coli</em> TOP10 F&rsquo; strain to prepare next  batch of competent cells.<br />
 +
                    Preparing  competent cells.<br />
 +
                    Isolation  of plasmid DNA from transformed <em>E.coli</em> (3C and 15L).<br />
 +
                    OD600&nbsp; of cell suspension (inoculated on  30.07.13).</p>
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                  <table border="1" cellspacing="0" cellpadding="0">
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                    <tr>
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                      <td width="80" valign="top"><br />
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                        Flask # </td>
 +
                      <td width="432" valign="top"><p>Part number.no of    colony form plate</p></td>
 +
                      <td width="256" valign="top"><p>OD600<strong></strong></p></td>
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                    </tr>
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                    <tr>
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                      <td width="80" valign="top"><p>1</p></td>
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                      <td width="432" valign="top"><p>15L.2</p></td>
 +
                      <td width="256" valign="top"><p>0,31</p></td>
 +
                    </tr>
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                    <tr>
 +
                      <td width="80" valign="top"><p>2</p></td>
 +
                      <td width="432" valign="top"><p>15L.3</p></td>
 +
                      <td width="256" valign="top"><p>0,30</p></td>
 +
                    </tr>
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                    <tr>
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                      <td width="80" valign="top"><p>3</p></td>
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                      <td width="432" valign="top"><p>15L.1</p></td>
 +
                      <td width="256" valign="top"><p>0,24</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="80" valign="top"><p>4</p></td>
 +
                      <td width="432" valign="top"><p>3C.1</p></td>
 +
                      <td width="256" valign="top"><p>0,32</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="80" valign="top"><p>5</p></td>
 +
                      <td width="432" valign="top"><p>3C.2</p></td>
 +
                      <td width="256" valign="top"><p>0,31</p></td>
 +
                    </tr>
 +
                  </table>
 +
                  <p>Week 4<br />
 +
                    Preparing <em>M. organophilum </em>cells to isolation of  genomic DNA.<br />
 +
                    Isolation of genomic DNA of <em>M.organophilum</em>.<br />
 +
                    Measuring  concentration of isolated DNA with NanoDrop &ndash; result not good enough for  performing PCR.<br />
 +
                    Inoculation  of medium with <em>M.organophilum</em> for  next isolation.<br />
 +
                    Isolation  of genomic DNA from <em>M.organophilum</em> with cold lysis buffer.<br />
 +
                    Results  measured with NanoDrop.</p>
 +
                  <table border="1" cellspacing="0" cellpadding="0">
 +
                    <tr>
 +
                      <td width="194" valign="top"><br />
 +
                        Probe nr </td>
 +
                      <td width="194" valign="top"><p>Concentration ng/&mu;l</p></td>
 +
                      <td width="194" valign="top"><p>260</p></td>
 +
                      <td width="194" valign="top"><p>280</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>1</p></td>
 +
                      <td width="194" valign="top"><p>278,8</p></td>
 +
                      <td width="194" valign="top"><p>1,89</p></td>
 +
                      <td width="194" valign="top"><p>1,75</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>2</p></td>
 +
                      <td width="194" valign="top"><p>355,8</p></td>
 +
                      <td width="194" valign="top"><p>1,82</p></td>
 +
                      <td width="194" valign="top"><p>1,82</p></td>
 +
                    </tr>
 +
                  </table>
 +
                  <p>Week 5<br />
 +
                    Running PCR  with previously isolated genomic DNA. <br />
 +
                    Running  agarose electrophoresis in search of PCR product. <br />
 +
  <img src="https://static.igem.org/mediawiki/2013/1/12/Attributions_clip_image003.jpg" alt="plik2" width="474" height="316" border="0" /> <br />
 +
                    In wells 5,  6 and 7 we can see a PCR product that we were aiming to have.<br />
 +
                    Isolation  of PCR product from gel with DNA purification kit. Measuring results with  NanoDrop &ndash; results were not good enough. Purification of PCR product from PCR  reaction mix. Measuring results with NanoDrop &ndash; results were not good enough.<br />
 +
                    Week 6<br />
 +
                    Isolation  of genomic DNA from <em>M.organophilum</em>.<br />
 +
                    Running PRC  with temperature gradient from isolated DNA. <br />
 +
  <img src="https://static.igem.org/mediawiki/2013/6/68/Attributions_clip_image005.jpg" alt="plik3" width="422" height="311" border="0" /> <br />
 +
                    Running gel  electrophoresis with PCR reaction mix. Purification of PCR product from gel.<br />
 +
                    Results:</p>
 +
                  <table border="1" cellspacing="0" cellpadding="0">
 +
                    <tr>
 +
                      <td width="194" valign="top"><br />
 +
                        No. of well </td>
 +
                      <td width="194" valign="top"><p>DNA concentration    ng/&mu;l</p></td>
 +
                      <td width="194" valign="top"><p>260</p></td>
 +
                      <td width="194" valign="top"><p>280</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>1</p></td>
 +
                      <td width="194" valign="top"><p>36</p></td>
 +
                      <td width="194" valign="top"><p>-</p></td>
 +
                      <td width="194" valign="top"><p>-</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>3</p></td>
 +
                      <td width="194" valign="top"><p>41,8</p></td>
 +
                      <td width="194" valign="top"><p>2,05</p></td>
 +
                      <td width="194" valign="top"><p>0,43</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>4</p></td>
 +
                      <td width="194" valign="top"><p>41,1</p></td>
 +
                      <td width="194" valign="top"><p>1,88</p></td>
 +
                      <td width="194" valign="top"><p>0,47</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>5</p></td>
 +
                      <td width="194" valign="top"><p>50,6</p></td>
 +
                      <td width="194" valign="top"><p>2,09</p></td>
 +
                      <td width="194" valign="top"><p>0,25</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>6</p></td>
 +
                      <td width="194" valign="top"><p>46,9</p></td>
 +
                      <td width="194" valign="top"><p>1,95</p></td>
 +
                      <td width="194" valign="top"><p>0,31</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>7</p></td>
 +
                      <td width="194" valign="top"><p>40,1</p></td>
 +
                      <td width="194" valign="top"><p>1,9</p></td>
 +
                      <td width="194" valign="top"><p>0,29</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="194" valign="top"><p>10</p></td>
 +
                      <td width="194" valign="top"><p>53,7</p></td>
 +
                      <td width="194" valign="top"><p>1,91</p></td>
 +
                      <td width="194" valign="top"><p>0,34</p></td>
 +
                    </tr>
 +
                  </table>
 +
                  <p>Week 7<br />
 +
                    Linear  backbone pSB1C3 digestion according to protocol provided by iGEM. <br />
 +
                    Ligation of  backbone with PCR product from well 10 &ndash; failed.<br />
 +
                    Ligation  with restriction enzymes from a different company &ndash; failed.<br />
 +
                    Week 8<br />
 +
                    Ligation  with restriction enzymes from yet another company &ndash; successful.<br />
 +
                    Transformation  of competent cells &ndash; failed.<br />
 +
                    Transformation  of competent cells with another batch of competent cells &ndash; successful. <br />
 +
                    Week 9<br />
 +
                    Isolation  of plasmid DNA.<br />
 +
                    Running  agarose electrophoresis to check if the plasmid contains insert &ndash; it does.<br />
 +
                    Sending a  BioBrick part to the registry.<br />
 +
                    Week 10<br />
 +
                    PCR: promoter with restriction sites suitable for cloning into pKT230 plasmid &ndash; successful.<br />
 +
                    Ligation of  PCR product with pKT230 plasmid &ndash; successful.</p>
 +
                  <p>&nbsp;</p>
 +
                  <h2>Protocols.<br />
 +
                    </h2>
 +
                  <h2>&nbsp;</h2>
 +
                  <p><strong>Chemical  transformation.</strong><br />
 +
                    Perform the same procedure for control test.</p>
 +
                  <ol>
 +
                    <li>Remove tube of frozen  competent cells from -70 C and place on ice. </li>
 +
                    <li>Remove 100ul per  transformation into a sterile pre-chilled Eppendorf tube. </li>
 +
                    <li>Add 25ng of DNA (2-10ul)  to the tube. Flick the tube several times. </li>
 +
                    <li>Leave the tube on ice  for at least 10 minutes.&nbsp; </li>
 +
                    <li>Heat shock the cells for  45s at&nbsp;42 C. </li>
 +
                    <li>Place tubes on ice for 2 minutes.&nbsp; </li>
 +
                    <li>Add 900ul of preheated  to 37&deg;C LB medium and incubate for 1 hour  at 37 C with shaking at 225 rpm. </li>
 +
                    <li>&nbsp;Plate 100ul of the cells onto antibiotic  plates. </li>
 +
                    <li>&nbsp;Place plates in the 37&deg;C incubator and grow overnight. </li>
 +
                  </ol>
 +
                  <p><strong>Preparation of  competent cells. </strong><br />
 +
                    1. Prepare 25ml  of sterile 50mM CaCl2 and cool it in a refrigerator.<br />
 +
  &nbsp;2. Innoculate one 1ml of LB medium with appropriate strain of E.coli. <br />
 +
                    3. Culture it  overnight in 37&deg;C.<br />
 +
                    4. Innoculate 40  ml of medium with overnight culture and culture it in 37&deg;C.<br />
 +
  &nbsp;5. When OD600 = 0,2 &ndash; 0,25 cool the culture on  ice for 15 minutes. <br />
 +
                    6. Centrifuge (5 000 rpm, 10 min, 4 &deg;C). <br />
 +
                    7. Suspend the  pellet in 20ml of cold CaCl2. <br />
 +
                    8. Incubate on ice for 20 minutes. <br />
 +
                    9. Centrifuge (5  000 rpm, 10 min, 4 &deg;C) .<br />
 +
                    10. Suspend the  pellet in 1ml of cold CaCl2. <br />
 +
                    11. Incubate for  30-40 minutes on ice.</p>
 +
                  <p>&nbsp;</p>
 +
                  <p><strong>Plasmid DNA isolation</strong> &ndash; according to a protocol  delivered with a kit (GenElute&trade;&nbsp;Plasmid  Miniprep Kit).</p>
 +
                  <p><strong>Genomic DNA isolation</strong> &ndash; according to a protocol  delivered with a kit (Wizard&reg; Genomic DNA Purification Kit).</p>
 +
                  <p><strong>Purification of DNA  from agarose gel and PCR mixture</strong> &ndash; according to a protocol delivered with a kit  (Wizard&reg; SV Gel and PCR Clean-Up System).</p>
 +
                  <p>&nbsp;</p>
 +
                  <p><strong>Agarose  electrophoresis &ndash; 2% gel.</strong></p>
 +
                  <p>1. Dissolve 1,2 agarose in 60 ml of 0,5xTBE buffer.  Heat the mixture up.</p>
 +
                  <p>&nbsp;2. When  cooled to about 60&deg;C, pour the mixture into the gel mold. Wait for it to cool  down.</p>
 +
                  <p>3. Mix the DNA sample with GelRed dye and loading  buffer. Load the sample and DNA ladder.</p>
 +
                  <p>4. Run the electrophoresis in 0,5xTBA, for 30 min,  under 60V.</p>
 +
                  <p>&nbsp;</p>
 +
                  <p><strong>PCR program for promoter with  BioBrick overhangs.</strong></p>
 +
                  <table border="1" cellspacing="0" cellpadding="0">
 +
                    <tr>
 +
                      <td valign="top"><br />
 +
                        Temperature </td>
 +
                      <td valign="top"><p>Time</p></td>
 +
                      <td valign="top"><p>Repeats</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>95&deg;C </p></td>
 +
                      <td valign="top"><p>3 min</p></td>
 +
                      <td valign="top"><p>X1</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>95&deg;C </p></td>
 +
                      <td valign="top"><p>30s</p></td>
 +
                      <td rowspan="3" valign="top"><p>X10</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p><strong>50&deg;C</strong><strong> </strong></p></td>
 +
                      <td valign="top"><p>45s</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>72&deg;C </p></td>
 +
                      <td valign="top"><p>45s</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>95&deg;C </p></td>
 +
                      <td valign="top"><p>30s</p></td>
 +
                      <td rowspan="3" valign="top"><p>X25</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p><strong>70&deg;C</strong><strong> </strong></p></td>
 +
                      <td valign="top"><p>45s</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>72&deg;C </p></td>
 +
                      <td valign="top"><p>45s</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>72&deg;C </p></td>
 +
                      <td valign="top"><p>2 min</p></td>
 +
                      <td valign="top"><p>X1</p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td valign="top"><p>4&deg;C </p></td>
 +
                      <td valign="top"><p>-</p></td>
 +
                      <td valign="top"><p>X1</p></td>
 +
                    </tr>
 +
                  </table>
 +
                  <p>Gradient of temperatures in  different PCR tubes (2 bolded values in the previous table):</p>
 +
                  <table border="1" cellspacing="0" cellpadding="0">
 +
                    <tr>
 +
                      <td width="92" valign="top"><br />
 +
                        A </td>
 +
                      <td width="111" valign="top"><p>53,7&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>79&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>B</p></td>
 +
                      <td width="111" valign="top"><p>53&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>77,2&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>C</p></td>
 +
                      <td width="111" valign="top"><p>51,8&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>74,2&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>D</p></td>
 +
                      <td width="111" valign="top"><p>50&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>70&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>E</p></td>
 +
                      <td width="111" valign="top"><p>47,6&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>64,4&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>F</p></td>
 +
                      <td width="111" valign="top"><p>46&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>60,4&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>G</p></td>
 +
                      <td width="111" valign="top"><p>44,6&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>57,2&deg;C </p></td>
 +
                    </tr>
 +
                    <tr>
 +
                      <td width="92" valign="top"><p>H</p></td>
 +
                      <td width="111" valign="top"><p>43,7&deg;C </p></td>
 +
                      <td width="111" valign="top"><p>55&deg;C </p></td>
 +
                    </tr>
 +
                  </table>
 +
                  <p><strong>PCR mix:</strong><br />
 +
                    12,5 ul of  MasterMix (GoTaq&reg; G2 Hot Start Master Mix)<br />
 +
                    0,5 ul of  1uM forward primer<br />
 +
                    0,5 ul of  1uM reverse primer<br />
 +
                    1 ul of  138ng/ul genomic DNA<br />
 +
                    10,5 ul  MiliQ water</p>
 +
                  <p>&nbsp;</p>
 +
                  <p>&nbsp;</p>
 +
                  <p>&nbsp;</p>
 +
                <p><strong>&nbsp;</strong></p></td>
 +
              </tr>
 +
            </table>
 +
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You should make use of the calendar feature on the wiki and start a lab notebook.  This may be looked at by the judges to see how your work progressed throughout the summer.  It is a very useful organizational tool as well.
 

Latest revision as of 16:41, 4 October 2013

Gdansk UG

Home Team

Official

Team Profile

Project

Parts Submitted

to the Registry
Human Practice Notebook Safety Attributions
 
 

Week 1
6 flasks were prepared with different alcohol concentration for determining M.organophilum tolerance to methanol, tolerance of aerobic conditions and tolerance to ethanol.
Medium used for cultivating M.organophilum contains:

  • 5g peptone
  • 3g meat extract
  • Distilled water to 1l
  • pH adjusted to 7.0
  • plik1

#

Content of flask

OD600 after 2 hours

OD600 
25.06.13

OD600
26.06.13

OD600
28.06.13.13

OD600
04.07.13

1

1% methanol

0,109

0,06

0,138

0,145

0,184

2

1% under layer of paraffin

0,06

0,071

0,117

0,155

0,461

3

2% methanol

0,055

0,066

0,086

0,210

0,450

4

1% ethanol

-0,08

0,078

0,047

0,073

0,071

5

2% ethanol

0,07

-0,013

0,047

0,067

0,079

6

5% ethanol

0,02

0,076

0,031

0,011

0,033

Week 2
Inoculating liquid medium with E.coli TOP10 F’ (in preparation for transformation).
OD600  of E.coli after one night – 0,718
Preparing competent E.coli TOP10 F’ cells.
Transformation of E.coli with iGEM Transformation efficiency Kit according to protocol provided by iGEM - http://parts.igem.org/Help:Transformation_Efficiency_Kit.
Transformation of E.coli TOP10 F’ cells with BioBricks:

  • BBa_K316003 – 3C in plate 1
  • BBa_K823017  - 3D in plate 1
  • BBa_K895006  - 15L in plate 1

Incubation in 37° C.
Transformation results:


Plasmid

Number of colonies

Control (without plasmid)

0

3C

2

3D

0

15L

4

Inoculation of plates with basic medium and 25mg/l chloramphenicol with colonies from 3C and 15L plate.
Week 3
Inoculation liquid medium with cholamphenicol (25mg/l) with 1 colony of transformed E.coli (3C and 15L).
 Inoculating liquid medium with E.coli TOP10 F’ strain to prepare next batch of competent cells.
Preparing competent cells.
Isolation of plasmid DNA from transformed E.coli (3C and 15L).
OD600  of cell suspension (inoculated on 30.07.13).


Flask #

Part number.no of colony form plate

OD600

1

15L.2

0,31

2

15L.3

0,30

3

15L.1

0,24

4

3C.1

0,32

5

3C.2

0,31

Week 4
Preparing M. organophilum cells to isolation of genomic DNA.
Isolation of genomic DNA of M.organophilum.
Measuring concentration of isolated DNA with NanoDrop – result not good enough for performing PCR.
Inoculation of medium with M.organophilum for next isolation.
Isolation of genomic DNA from M.organophilum with cold lysis buffer.
Results measured with NanoDrop.


Probe nr

Concentration ng/μl

260

280

1

278,8

1,89

1,75

2

355,8

1,82

1,82

Week 5
Running PCR with previously isolated genomic DNA.
Running agarose electrophoresis in search of PCR product.
plik2
In wells 5, 6 and 7 we can see a PCR product that we were aiming to have.
Isolation of PCR product from gel with DNA purification kit. Measuring results with NanoDrop – results were not good enough. Purification of PCR product from PCR reaction mix. Measuring results with NanoDrop – results were not good enough.
Week 6
Isolation of genomic DNA from M.organophilum.
Running PRC with temperature gradient from isolated DNA.
plik3
Running gel electrophoresis with PCR reaction mix. Purification of PCR product from gel.
Results:


No. of well

DNA concentration ng/μl

260

280

1

36

-

-

3

41,8

2,05

0,43

4

41,1

1,88

0,47

5

50,6

2,09

0,25

6

46,9

1,95

0,31

7

40,1

1,9

0,29

10

53,7

1,91

0,34

Week 7
Linear backbone pSB1C3 digestion according to protocol provided by iGEM.
Ligation of backbone with PCR product from well 10 – failed.
Ligation with restriction enzymes from a different company – failed.
Week 8
Ligation with restriction enzymes from yet another company – successful.
Transformation of competent cells – failed.
Transformation of competent cells with another batch of competent cells – successful.
Week 9
Isolation of plasmid DNA.
Running agarose electrophoresis to check if the plasmid contains insert – it does.
Sending a BioBrick part to the registry.
Week 10
PCR: promoter with restriction sites suitable for cloning into pKT230 plasmid – successful.
Ligation of PCR product with pKT230 plasmid – successful.

 

Protocols.

 

Chemical transformation.
Perform the same procedure for control test.

  1. Remove tube of frozen competent cells from -70 C and place on ice.
  2. Remove 100ul per transformation into a sterile pre-chilled Eppendorf tube.
  3. Add 25ng of DNA (2-10ul) to the tube. Flick the tube several times.
  4. Leave the tube on ice for at least 10 minutes. 
  5. Heat shock the cells for 45s at 42 C.
  6. Place tubes on ice for 2 minutes. 
  7. Add 900ul of preheated to 37°C LB medium and incubate for 1 hour at 37 C with shaking at 225 rpm.
  8.  Plate 100ul of the cells onto antibiotic plates.
  9.  Place plates in the 37°C incubator and grow overnight.

Preparation of competent cells.
1. Prepare 25ml of sterile 50mM CaCl2 and cool it in a refrigerator.
 2. Innoculate one 1ml of LB medium with appropriate strain of E.coli.
3. Culture it overnight in 37°C.
4. Innoculate 40 ml of medium with overnight culture and culture it in 37°C.
 5. When OD600 = 0,2 – 0,25 cool the culture on ice for 15 minutes.
6. Centrifuge (5 000 rpm, 10 min, 4 °C).
7. Suspend the pellet in 20ml of cold CaCl2.
8. Incubate on ice for 20 minutes.
9. Centrifuge (5 000 rpm, 10 min, 4 °C) .
10. Suspend the pellet in 1ml of cold CaCl2.
11. Incubate for 30-40 minutes on ice.

 

Plasmid DNA isolation – according to a protocol delivered with a kit (GenElute™ Plasmid Miniprep Kit).

Genomic DNA isolation – according to a protocol delivered with a kit (Wizard® Genomic DNA Purification Kit).

Purification of DNA from agarose gel and PCR mixture – according to a protocol delivered with a kit (Wizard® SV Gel and PCR Clean-Up System).

 

Agarose electrophoresis – 2% gel.

1. Dissolve 1,2 agarose in 60 ml of 0,5xTBE buffer. Heat the mixture up.

 2. When cooled to about 60°C, pour the mixture into the gel mold. Wait for it to cool down.

3. Mix the DNA sample with GelRed dye and loading buffer. Load the sample and DNA ladder.

4. Run the electrophoresis in 0,5xTBA, for 30 min, under 60V.

 

PCR program for promoter with BioBrick overhangs.


Temperature

Time

Repeats

95°C

3 min

X1

95°C

30s

X10

50°C

45s

72°C

45s

95°C

30s

X25

70°C

45s

72°C

45s

72°C

2 min

X1

4°C

-

X1

Gradient of temperatures in different PCR tubes (2 bolded values in the previous table):


A

53,7°C

79°C

B

53°C

77,2°C

C

51,8°C

74,2°C

D

50°C

70°C

E

47,6°C

64,4°C

F

46°C

60,4°C

G

44,6°C

57,2°C

H

43,7°C

55°C

PCR mix:
12,5 ul of MasterMix (GoTaq® G2 Hot Start Master Mix)
0,5 ul of 1uM forward primer
0,5 ul of 1uM reverse primer
1 ul of 138ng/ul genomic DNA
10,5 ul MiliQ water