<p><b>Results Miniprep: </b>

                                      <strong>Sample Name</strong>

                                  </p>

                          </tr>

                          <tr>

                                      -

                                      -

                                  <p>

                                      <strong>BBa_K1058008</strong>

                                  </p>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                                  <p align="center">

                          </tr>

                   </p>

                   <p><b>Results Sequencing: </b><a data-toggle="modal" data-target="#BBa_K1058008-figure1-modal" class="journal-protocol"> Figure 1 </a></p>

                   <p><b>Next Steps:</b> PCR of parts of <a href="http://parts.igem.org/Part:BBa_K1058008">BBa_K1058008</a>.</p>

        </div>

    </div>

  </div>

  </div>

<!-- WEEK 2 -->

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    <div class="box">

        <div class="labtitle">29/06 - 05/07</div>

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          <div class="box-content">

          <p class="journal-summary-heading">Summary</p>

        <p class="journal-content"> During this week, <a href="http://parts.igem.org/Part:BBa_K1058008" target="_blank">BBa_K1058008</a> was disassembled into its constituent parts, pChr, and ChrB.</p>

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        <!-- when copying for next week, make sure to change labtitle, span, collapsible in last line. In each separate day change span and following div-->

             <span class="box-title">Day 1</span> <!--Title of collapsible box-->

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                   <p><b>Aim of experiment: </b> To break down <a href="http://parts.igem.org/Part:BBa_K1058008" target="_blank">BBa_K1058008</a> into the promoter region pChr, and the repressor gene, ChrB, while adding standard prefix and suffix to each. Furthermore optimisation of first 15 codons of ChrB in order to increase the overall rate of transcription. Restriction digest of the respective ends and subsequent ligation of pChr and ChrB into pSB1C3 for submission to registry.</p>

                     <p><a data-toggle="modal" data-target="#PCR-modal" class="journal-protocol"> Click here to see our PCR protocol.</a></p>

                     <p><a data-toggle="modal" data-target="#gelextraction-modal" class="journal-protocol"> Click here to see our gel extraction protocol.</a></p>

                  </p>

                   <p><b>Results:</b>

                  <p><a data-toggle="modal" data-target="#dundee15-chr-igem022-modal" class="journal-protocol"> Figure 2: Agarose gel after PCR of pChr and ChrB. </a></p>

                  <p>As can be seen on the image of the gel, PCR of ChrB was not successful. pChr was further processed by restriction digest with EcoRI and PstI</p></p>

                   <p><b>Next Steps:</b> Repeat of PCR of ChrB. Purification of the Plasmid, containing <a href="http://parts.igem.org/Part:BBa_K1058008">BBa_K1058008</a> and confirmation of size and sequence.</p>

<!-- WEEK 3 -->

         <div class="labtitle">06/07 - 12/07</div>

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         <p class="journal-content">During this week ligations of pChr and ChrB into pSB1C3 were finalised and the constituent parts of our newly designed chromate sensing system were prepared for ligation and transformation.</p>

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                   <p><b>Aim of experiment:</b> To repeat PCR of ChrB for subsequent ligation into pSB1C3. Ligation of pChr and ChrB into pSB1C3. Transformation of each into a non-pathogenic lab strain of E. coli.

                  <p>Overnight culture of strain, containing GFPmut2, as a fluorescent reporter for our Chromate sensing system</p></p>

                     <p><a data-toggle="modal" data-target="#PCR-modal" class="journal-protocol"> Click here to see our PCR protocol.</a> <p>The annealing temperature was lowered in order to increase the chances of accomodating a primer that is not 100% complementary. Furthermore different concentrations of DMSO were tested.</p></p>

                    <p><a data-toggle="modal" data-target="#ligation-modal" class="journal-protocol"> Click here to see our ligation protocol.</a> Ligations were made in 2:1 and 3:1 ratio.</p>

                     <p><a data-toggle="modal" data-target="#overnightculture-modal" class="journal-protocol"> Click here to see our Overnight culture protocol.</a></p>

                  </p>

                   <p><b>Results:</b>

                   <p><a data-toggle="modal" data-target="#dundee15-chr-igem023-modal" class="journal-protocol"> Figure 3: Agarose gel after PCR of ChrB. </a></p>  

                   <p>pChr, ChrBs, and ChrBw were ligated into pSB1C3.</p>

                  <p>pChr-pSB1C3, ChrBs-pSB1C3, and ChrBw-pSB1C3 were transformed into E. coli MC1061.</p></p>

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                   <p><b>Aim of experiment:</b> Purification of GFPmut2 from overnight cultures. Overnight cultures of recombinant MC1061, containing pChr-pSB1C3, ChrBs-pSB1C3, and ChrBw-pSB1C3 respectively. Overnight culture of pUniprom for subsequent ligation of ChrB</p>

                     <p><a data-toggle="modal" data-target="#miniprep-modal" class="journal-protocol"> Miniprep</a> for plasmid purification of overnight culture of GFPmut2.</p>

                    <p><a data-toggle="modal" data-target="#PCR-modal" class="journal-protocol"> PCR</a> for amplification of GFPmut2 and ChrB.</p>

                    <p><a data-toggle="modal" data-target="#gelextraction-modal" class="journal-protocol"> Gel extraction</a> of PCR product pf GFPmut2.</p>

                     <p><a data-toggle="modal" data-target="#overnightculture-modal" class="journal-protocol"> Overnight culture</a> of MC1061 containing pChr-pSB1C3, ChrBs-pSB1C3, and ChrBw-pSB1C3 respectively. Furthermore of a strain containing the vector pUniprom.</p>

                  </p>

                   <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-igem024-modal" class="journal-protocol"> Figure 5 </a> Since amplification of ChrB was unsuccessful, it will be repeated.</p>

                   <p><b>Next Steps:</b> Sequence and size confirmation of pChr-pSB1C3, ChrBs-pSB1C3, and ChrBw-pSB1C3.</p>

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                   <p><b>Aim of experiment:</b> To purify overnight cultures for size and sequence confirmation. Repeat of PCR amplification of pChr and ChrB. Restriction digestes of all parts in order to produce compatible sticky ends.</p>

                     <p><a data-toggle="modal" data-target="#miniprep-modal" class="journal-protocol"> Miniprep</a> of pChr-pSB1C3, ChrBs-pSB1C3, ChrBw-pSB1C3 and pUniprom.</p></p>

                                  <p>

                                      <strong>Blank</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                                  </p>

                              </td>

                          </tr>

                          <tr>                            

                              <td width="140" valign="top">

                                  <p>

                                      <strong>pUniprom2</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                              <td width="111" valign="top">

                          </tr>

                                  <p>

                                      <strong>pChr2</strong>

                                  </p>

                              </td>

                                      110.13

                                  </p>

                              </td>

                                  </p>

                          </tr>

                                  <p>

                                      <strong>pChr3</strong>

                                  </p>

                              <td width="111" valign="top">

                                  <p align="center">

                                      114.65

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                          </tr>

                                  <p>

                                      <strong>pChr4</strong>

                                  </p>

                              </td>

                                  <p align="center">

                          </tr>

                          <tr>

                                  <p>

                                      <strong>ChrBs2</strong>

                                  </p>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                                  <p align="center">

                          </tr>

                          </tr>

                                  <p>

                                      <strong>ChrBw1</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                      116.26

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                      ng/µl

                                  </p>

                              </td>

                          </tr>

                          <tr>

                              <td width="140" valign="top">

                                  <p>

                                      <strong>ChrBw3</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                              <td width="111" valign="top">

                          </tr>

                      </tbody>

                    </table>

                  </p>

                    <p><b>Protocols Used:</b>

                    <p><a data-toggle="modal" data-target="#PCR-modal" class="journal-protocol"> PCR</a> for amplification of pChr and ChrB.</p></p>

                    <p><a data-toggle="modal" data-target="#restriction_digest-modal" class="journal-protocol">Restriction digest</a> for confirmation of size of pChr and ChrB.</p></p>

                   <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-igem026-modal" class="journal-protocol"> Figure 6 </a> Agarose gel for size confirmation.</p>

 

                   <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-pChr1-modal" class="journal-protocol"> Figure 7 </a> Confirmed sequence of pChr1.</p>

                  <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-ChrBw4-modal" class="journal-protocol"> Figure 8 </a> Confirmed sequence of ChrBw4.</p>

 

                    <p><a data-toggle="modal" data-target="#restriction-digest-modal" class="journal-protocol"> Restriction digest</a> of gel purified PCR-products of pChr, ChrB, and GFPmut2, using EcoRI/SpeI, BamHI/HindIII, and XbaI/PstI respecitvely.</p></p>

             <span class="box-title">Day 4</span> <!--Title of collapsible box-->

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                   <p><b>Aim of experiment:</b> To prepare pUniprom for insertion of ChrB.</p>

                     <p><a data-toggle="modal" data-target="#restriction-digest-modal" class="journal-protocol">Restriction digest</a> of pUniprom with BamHI and HindIII.</p>

                     <p><a data-toggle="modal" data-target="#gel-extraction-modal" class="journal-protocol">Gel extraction</a> of digested pUniprom</p>

                  </p>

                   <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-igem034-modal" class="journal-protocol"> Figure 9 </a></p>

                   <p><b>Next Steps:</b> Ligation of ChrB into pUniprom.</p>

                   <p><b>Protocols Used:</b>

                    <p><a data-toggle="modal" data-target="#PCR-modal" class="journal-protocol">PCR</a> of optimised ChrB from the sequence confirmed ChrBw4-pSB1C3, adding restriction sites compatible to pUniprom.</p>

                    <p><a data-toggle="modal" data-target="#gelextraction" class="journal-protocol">Gel extraction</a> of optimised ChrBafter PCR.</p>

 

                  <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-igem034-modal" class="journal-protocol"> Figure 10 </a></p>

 

 

                  <p><b>Next Steps:</b> Ligation of ChrB and codon optimised ChrB into pUniprom.</p>

             <span class="box-title">Day 5</span> <!--Title of collapsible box-->

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                   <p><b>Aim of experiment:</b> Ligation of ChrB and optimised ChrB into pUniprom. Ligation of pChr and GFPmut2 into pSB1C3</p>

                     <p><a data-toggle="modal" data-target="#ligation-modal" class="journal-protocol">Ligation</a> of ChrB and optimised ChrB into pUniprom via BamHI and HindIII restriction sites. Ligation of pChr to GFPmut2 via Spe/Xba link and ligation of pChrGFP construct into pSB1C3 EcoRI/PstI restriction sites.</p>

                  </p>

                   <p><b>Next Steps:</b>Transformation of abovementioned ligations.</p>

<!-- WEEK 4 -->

         <div class="labtitle">13/07 - 19/07</div>

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         <p class="journal-content">During this week successful transformations were identifeid and propagated.></p>

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                   <p><b>Aim of experiment:</b> Transform recombinant vectors into E. coli chassis.</p>

                     <p><a data-toggle="modal" data-target="#transformation-modal" class="journal-protocol">Transformation</a> of ChrB-pUniprom, optimised ChrB-pUniprom and pChr-GFPmut2-pSB1C3 into JM110.</p>

                  </p>

                   <p><b>Results:</b><a data-toggle="modal" data-target="#dundee15-chr-first-transformation-modal" class="journal-protocol"> Figure 11 </a></p>

                   <p><b>Aim of experiment:</b> Backup of digested pSB1C3 for the case that a ligation with 2 inserts does not work.</p>

                     <p><a data-toggle="modal" data-target="#restriction-digest-modal" class="journal-protocol">Restriction digest</a> of pSB1C3 with EcoRI/SpeI for subsequent insertion of pChr.</p>

                  </p>

                   <p><b>Results:</b>N/A</p>

                   <p><b>Next Steps:</b> Store digested plasmid at -20^oC.</p>

             <span class="box-title">Day 2</span> <!--Title of collapsible box-->

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                   <p><b>Aim of experiment:</b> Purification of recombinant vectors for sequence and size confirmation.</p>

                     <p><a data-toggle="modal" data-target="#overnightculture-modal" class="journal-protocol"> Overnight culture</a> of JM110 with ChrB-pUniprom, optimised ChrB-pUniprom and pChr-GFPmut2-pSB1C3.</p>

                  <p><a data-toggle="modal" data-target="#plating-modal" class="journal-protocol"> Patch plating</a> of the same colonies.</p>

                  </p>

                   <p><b>Next Steps:</b> Purification of the recombinant plasmids for confirmation of size and sequence.</p>

             <span class="box-title">Day 3</span> <!--Title of collapsible box-->

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                 <div id="collapsiblew4-3" class="collapse box-content">

                   <p><b>Aim of experiment:</b> Purification of recombinant plasmids for confirmation of size and sequence.</p>

                     <p><a data-toggle="modal" data-target="#miniprep-modal" class="journal-protocol">Miniprep</a> of ChrB-pUniprom, optimised ChrB-pUniprom and pChr-GFPmut2-pSB1C3.</p>

                  </p>

                   <p><b>Results:</b>

                                  <p align="center">

                                      <strong>Sample Name</strong>

                                  </p>

                              <td width="111" valign="top">

                                  <p align="center">

                                      <strong>Concentration</strong>

                                  </p>

                          </tr>

                                      -

                                      -

                          </tr>

                                  <p>

                                      <strong>pSB1C3-pChr-GFPmut2_2</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                      355.31

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                      ng/µl

                                  </p>

                              </td>

                          </tr>

                          <tr>

                              <td width="140" valign="top">

                                  <p>

                                      <strong>pSB1C3-pChr-GFPmut2_4</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                              <td width="111" valign="top">

                          </tr>

                                  <p>

                                      <strong>pUniprom-ChrB-opt_2</strong>

                                  </p>

                              </td>

                                      214.17

                                  </p>

                              </td>

                                  </p>

                          </tr>

                                  <p>

                                      <strong>pUniprom-ChrB-opt_3</strong>

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                      140.85

                                  </p>

                              </td>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                          </tr>

                                  <p>

                                      <strong>pUniprom-ChrB-opt_4</strong>

                                  </p>

                              </td>

                                  <p align="center">

                          </tr>

                          <tr>

                                      <strong>pUniprom-ChrB_1</strong>

                                  <p>

                                      <strong>pUniprom-ChrB_2</strong>

                                  </p>

                              <td width="111" valign="top">

                                  <p align="center">

                                  </p>

                              </td>

                                  <p align="center">

                          </tr>

                                      <strong>pUniprom-ChrB_3</strong>

                          </tr>

                      </tbody>

                    </table>

                   </p>

                <p><b>Protocols Used:</b>

                    <p><a data-toggle="modal" data-target="#restriction-digest-modal" class="journal-protocol">Restriction digest</a> of ChrB-pUniprom and optimised ChrB-pUniprom with BamHI and HindIII. Restriction digest of pChr-GFPmut2-pSB1C3 with EcoRI/PstI.</p>

                  </p>

                     <p><a data-toggle="modal" data-target="#colony-modal" class="journal-protocol">Colony PCR</a> of pUniprom-ChrB-opt for elucidation of insert size or presence of insert.</p>

                  </p>