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-<h1> July </h1>
+<h1> Journal</h1>
-<h2> Week 3 </h2>
+<h2> July </h2>
+</html>{{:Team:UGent/Templates/ToggleBoxStart}}Week 4: july 22 - 28  {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
 <ul>
 <li> Introduction given by our lab instructors</li>
@@ Line 12: / Line 15: @@
 <li> General preparations: sterile mQ, sterile eppendorf </li>
 </ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}<html>
-<h1> August </h1>
+<h2> August </h2>
-<h2> Week 1 </h2>
+</html>{{:Team:UGent/Templates/ToggleBoxStart}}Week 1: july 29 - august 4  {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 2: august 5 - 11  {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
 <ul>
 <li> Experiment 1 </li>
 <ul class="a">
-<li> <b>Purify plasmid</b> pTGD-ccdA-Pmb1GFP-CmFRT using Qiagen spin mini kit: Nanodrop -- <b>362.4 ng/µL</b> </li>
+<li> <b>Inoculate</b> <i> E. coli </i>DH5a + pTGD-<i>ccdA</i>-Pmb1GFP-CmFRT </li>
-<li> <b>Preparative Restriction Digest (RD)</b> of purified plasmid: BspHI & BstAPI: expected fragments of <b>5541bp and 903 bp </b></li>
+<li> <b>Purify plasmid pTGD-<i>ccdA</i>-Pmb1GFP-CmFRT</b> using Qiagen spin mini kit: Nanodrop -- <b>362.4 ng/µL</b> </li>
-<li> <b>Gel purify RD-fragment of 5541 bp </b> using Qiagen Qiaquick gel extraction kit: Nanodrop -- <b>70.4 ng/µL</b></li>
+<li> <b>Preparative Restriction Digest (RD)</b> of purified plasmid: BspHI & BstAPI: expected fragments of 5541bp and 903 bp </li>
-<li> HiFi <B>PCR using Primestar polymerase</B> on RD (HR-ccdA-Pmb1GFP-HR)and on plasmid pTGD-ccdA-PMbAFGP-CmFRT  with MDM588 & MDM589. Analytical gel: <b>negative </b></li>
+<li> <b>Gel purify RD-fragment of 5541 bp</b> using Qiagen Qiaquick gel extraction kit: Nanodrop -- <b>70.4 ng/µL</b></li>
-<li> <b>PCR using Q5 polymerase </b> on RD (HR-ccdA-Pmb1GFP-HR)and on plasmid pTGD-ccdA-PMbAFGP-CmFRT  with MDM588 & MDM589. Analytical gel: <b> negative </b></li>
+<li> <b>PCR on RD (HR-<i>ccdA</i>-Pmb1GFP-HR)and on plasmid pTGD-<i>ccdA</i>-PMbAFGP-CmFRT  with MDM588 & MDM589</b>
-<li> PCR using Roche on RD (HR-ccdA-Pmb1GFP-HR)and on plasmid pTGD-ccdA-PMbAFGP-CmFRT  with MDM588 & MDM589. Analytical gel: <b> negative </b></li>
+<BR> ->HiFi PCR using Primestar polymerase. Analytical gel: <b>negative </b>
-<li> Touchdown PCR using Q5 polymerase on RD (HR-ccdA-Pmb1GFP-HR)and on plasmid pTGD-ccdA-PMbAFGP-CmFRT  with MDM588 & MDM589. Analytical gel: <b> negative </b></li>
+<BR> ->PCR using Q5 polymerase. Analytical gel: <b> negative </b>
-<li> Control plasmid pTGD-ccdA-PMbAFGP-CmFRT: RD with AclI. Expected fragments:.............. Analytical gel: <b> negative </b> --> <u> Problem with plasmid pTGD-ccdA-PMbAFGP-CmFRT </u></li>
+<BR> ->PCR using Roche. Analytical gel: <b> negative </b>
-<li> <b> Transformation</b>: Knock in with lineair DNA by electroporation. Incubation of the transformed cells and transfer the culture on a Cm plate. </li>
+<BR> ->Touchdown PCR using Q5 polymerase. Analytical gel: <b> negative </b> </li>
-<li> Colony PCR on 48 colonies using crimson taq polymerase with two primer pairs: MDM0141/MDM0010 and MDM0046/MDM123. Expected fragments: 550bp & 2450 bp. Analytic gel: <b> 4 positives </b> </li>
+<li> <b>Control plasmid pTGD-<i>ccdA</i>-PMbAFGP-CmFRT: RD with AclI.</b> Expected fragments: 758 bp, 1730 bp and 3956 bp. Analytical gel: <b> negative </b> --> <u> Problem with plasmid pTGD-<i>ccdA</i>-PMbAFGP-CmFRT </u></li>
+<li> <b> Transformation</b>: Knock in with <u>linear back-up</u> DNA by electroporation. Incubation of the transformed cells and transfer the culture on a Cm plate. </li>
+<li> Colony PCR on 48 colonies using crimson taq polymerase with two primer pairs: MDM0141/MDM0010 and MDM0046/MDM123. Expected fragments: 550bp & 2450 bp. Analytic gel: <b> 4 positives </b>
+<img src="https://static.igem.org/mediawiki/2013/0/02/UGent_2013_CPCR_KI.jpg" width="300"/></a></li>
 <li> Colony PCR on 4 positive and 4 negative colonies using crimson taq polymerase with out primers: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> negative </b>.</li>
 <li> 2 Colony PCR on 4 positive and 4 negative colonies using Taq and Phire polymerase with out primers: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> negative </b>.</li>
-<li> Colony PCR on 4 positive and 4 negative colonies using Emerald polymerase with out primers: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> 1 positive: colonie 35 </b>.</li>
+<li> Colony PCR on 4 positive and 4 negative colonies using Emerald polymerase with out primers: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> 1 positive: colonie 35 </b>.
+<img src="https://static.igem.org/mediawiki/2013/3/35/UGent_2013_CPCR_KI_out.png" width="200"/></a></li>
 </ul>
 <BR>
 <li> Experiment 2 </li>
 <ul class="a">
-<li> Inoculate <i>E.Coli</i> DH5a + p5SpFRT-T7ccdB <BR> Inoculate <i>E.Coli</i> DH5a + p10SpFRT-T7ccdB <BR> Inoculate <i>E.Coli</i> DH5a + p20SpFRT-T7ccdB </li>
+<li> Inoculate <i>E. coli</i> DH5a; + p5SpFRT-T7<i>ccdB</i> <BR> Inoculate <i>E. coli</i> DH5a; + p10SpFRT-T7<i>ccdB</i> <BR> Inoculate <i>E. coli</i> DH5a; + p20SpFRT-T7<i>ccdB</i> </li>
-<li> Purify plasmid pTGD-ccdA-Pmb1GFP-CmFRT using Qiagen spin mini kit: nanodrop <BR> p5SpFRT-T7ccdB: 119,6 ng/µl <BR> p10SpFRT-T7ccdB: 156,3 ng/µl <BR> p20SpFRT-T7ccdB: 392,9 ng/µl </li>
+<li> Purify plasmids using Qiagen spin mini kit: nanodrop <BR> p5SpFRT-T7<i>ccdB</i>: 119.6 ng/µl <BR> p10SpFRT-T7<i>ccdB</i>: 156.3 ng/µl <BR> p20SpFRT-T7<i>ccdB</i>: 392.9 ng/µl </li>
-<li> <b>CcdB operon</b>: HiFi PCR of plasmids p5SpFRT-T7ccdB, p10SpFRT-T7ccdB and p20SpFRT-T7ccdB with MDM0586/MDM0587 to amplify ccdB operon </li>
+<li> <b>CcdB operon</b>:
-<li> <B>Vector pSB4A5</B>:
+<br> -> HiFi PCR of plasmids p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i>ccdB</i> with MDM0586/MDM0587 to amplify <i>ccdB</i> operon
-<BR> -> Resuspend plasmid pSB4A5 from the iGEM kit (plate 5, well1)
+<br> -> Purification of CcdB operon PCR fragment using Qiagen Qiaquick PCR purification kit and checked on analytical gel (expected fragment of 2300 bp): nanodrop
-<BR> -> Transorm in <i> E.Coli </i> Top10 subcloning cells using heat shock
+<br> p5: 174.6 ng/µl
-<BR> -> Plate on ampicillin plate and grow overnight at 37°C </li>
+<br> p10: 24.5 ng/µl (consistent with small band on the analytival gel)
+<br> p20: 104.3 ng/µl
+<br> -> Redo of inoculation <i>E. coli</i> DH5a + p5SpFRT-T7<i>ccdB</i>, <i>E. coli</i> DH5a + p10SpFRT-T7<i>ccdB</i> and <i>E. coli</i> DH5a + p20SpFRT-T7<i>ccdB</i>
+<br> -> Redo of purification of plasmids p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i>ccdB</i> using Qiagen Spin minikit: nanodrop <BR> p5SpFRT-T7<i>ccdB</i>: 21.1 ng/µl <BR> p10SpFRT-T7<i>ccdB</i>: 25.1 ng/µl <BR> p20SpFRT-T7<i>ccdB</i>: 24.6 ng/µl
+</li>
+</li>
+<li> <B>Vectors pSB4A5</B> (plate 5, well 5I), <B>pSB3T5</B> (plate 2, well 8D) and <B>pSB6A1</B> (plate 2, well 2L)</B>:
+<BR> -> Resuspend plasmids from the iGEM kit
+<BR> -> Transform in <i>E. coli </i> Top10 subcloning cells using elektroporation
+<BR> -> Plate pSB4A5 and pSB6A1 on ampicillin plate and pSB3T5 on tetracyclin
+and grow overnight at 37°C
+<BR> -> Plates with transformants: pSB6A1 lots of colonies, pSB3T5 sufficient colonies and pSB4A5 no colonies
+</li>
+<li> <B>Vectors pSB4A5 </B>(plate 5, well 5I):
+<BR> -> Resuspend plasmids from the iGEM kit
+<BR> -> Transform in <i>E. coli</i> Top10 subcloning cells using elektroporation
+<BR> -> Plate on ampicillin plate and grow overnight at 37°C (1 plate 150 µl, 1 plate 50 µl)
+<BR> -> Plates with transformants: pSB4A5 no colonies</li>
+<li>Inoculation colonies of pSB3T5 and pSB6A1 -> at the end of the day replaced from 37°C to 30°C</li>
+<li><b>Vector pSB4A5 </b>(plate 5, well 1I and plate 2, well 2J as backup) and <b>pSB6A1 </b>(plate 5, well 1K as backup):
+<BR> -> Resuspend plasmid pSB4A5 and pSB6A1 from the iGEM kit
+<BR> -> Transform in <i>E. coli</i> Top10 subcloning cells (heat shock)
+<BR> -> Plate transformation on ampicillin plate and grow overnight at 37°C (3 plates: 10<sup>-2</sup>,10<sup>-1</sup> and 10<sup>0</sup>)
+<BR> -> Plates with transformants: pSB4A5 (plate 2, well 2J) colonies, pSB4A5 (plate 5, well 1I) no colonies and pSB6A1 (plate 2, 2L) few colonies
+</li>
+<li> Inoculate pSB3T5 and pSB6A1  again and in warm chamber (37°C). </li>
+<li> Inoculation colonies of pSB4A5 (plate 2, well 2J) and pSB6A1 (plate 2, well 2L) (2 times: one for further work and one for cryovials)
+<li> Purification of plasmids pSB3T5, pSB6A1 and pSB4A5 </li>
+<li> Generation of <b>restriction</b> digest fragments of T7-<i>ccdB</i> insert (from p5SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i>ccdB</i>) and vector (pSB3T5 (2x), pSB4A5 (from plate 2, well 2J) and pSB6A1 (1x from plate 5, well 1K and 1x from plate 2, well 2L) with XbaI and PstI-HF (gel purify RD-fragments using Qiagen Qiaquick gel extraction kit (expected fragment of 2157 bp for T7-<i>ccdB</i>, 3229 bp for pSB3T5, 3372 bp for pSB4A5 and 3999 bp for pSB6A1): Nanodrop
+<br>p5: 43.7 ng/µl
+<br>p20: 24.2 ng/µl
+<br>pSB3T5 (inoculation 1): 23.5 ng/µl
+<br>pSB3T5 (inoculation 2): 23 ng/µl
+<br>pSB4A5: 40.5 ng/µl
+<br>pSB6A1 (plate 2, 2L): 40.1 ng/µl
+<br>pSB6A1 (plate 5, 1K): 30.4 ng/µl </li>
+<li> <b>Ligation</b> of T7-<i>ccdB</i> from p5SpFRT-T7<i>ccdB</i> and pSB6A1 (1x from plate 5, well 1K and 1x from plate 2, well 2L), p20SpFRT-T7<i>ccdB</i> and pSB3T5, p20SpFRT-T7<i>ccdB</i> and pSB4A5 (from plate 2, well 2J)  (3(insert)/1(plasmid) ratio) </li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 (heat shock)</li>
+<li> Plate transformation on ampicillin (pSB4A5 and pSB6A1) and tetracycline plate (pSB3T5) and grow overnight at 37°C (2 plates: 10<sup>-2</sup>, 10<sup>-1</sup>)
+<br> -> Plates with transformants: no colonies</li>
+<li> New <b>transformation</b> in <i>E. coli</i> Top10 from pSB4A5 and pSB6A1 using heat shock
+<br> -> Plates with transformants: pSB6A1 2 colonies, pSB4A5 few colonies </li>
+<li> New <b>ligation</b> with RD-fragments created before (vectors pSB3T5, pSB4A5, pSB6A1 (plate 5, well 1K) and insert T7-<i>ccdB</i> created in experiment 6), at 22.5°C o/n) </li>
+<li> <b>CcdB operon</b>:
+<br> -> HiFi PCR of plasmids p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i><i>ccdB</i></i> with MDM0586 & MDM0587 to amplify <i>ccdB</i> operon </li>
 </ul>
 <br>
 <li> Experiment 6 </li>
+<ul class="a">
+<li> <b>CcdB operon</b>:
+<br> -> HiFi PCR of plasmids p20SpFRT-T7<i>ccdB</i> with MDM0586/MDM0587 to amplify <i>ccdB</i> operon
+<br> nanodrop: 301,5 ng/µl </li>
+<li> <b>Vector pSB1C3</b> (plate 1, well 23O):
+<BR> -> Resuspend plasmids from the iGEM kit
+<br> -> Transform pSB1C3 in <i>E. coli</i> Top10 subcloning cells, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C
+<br> -> Inoculate <i>E. coli</i> Top10 + pSB1C3
+<br> -> Purify plasmids using Qiagen Qiaprep Spin minikit: nanodrop: 200,2 ng/µl</li>
+<li> <b>Restriction</b> of CcdB operon and pSB1C3 with XbaI and PstI
+<br> Preparative gel:  <img src="https://static.igem.org/mediawiki/2013/9/90/Preparatieve_gel_week2_aug.jpg" width="100"/></a>
+<br> restriction digest of T7-<i>ccdB</i> (expected to be 2044bp) and restriction digest of backbone of pSB1C3 (expected length is 2232 bp)
+<br> -> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br> Restriction digest of T7-<i>ccdB</i>: 16.9 ng/µl
+<br> Restriction digest of pSB1C3: 12.3 ng/µl</li>
+<li> <b>Ligation</b> of CcdB operon and pSB1C3</li>
+<li> <b>Transformation</b> in <i> E. coli </i> Top10 subcloning cells, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>negative</b>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 3: august 12 - 18   {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 1 </li>
+<ul class="a">
+<li>Inoculation positive colonie on cm plate. </li>
+<li>Colony PCR on 8 kolonies using emerald polymerase with out primers: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> positive: 5 & 8 </b>.<br>
+<img src="https://static.igem.org/mediawiki/2013/8/85/CPCR_KI_out2.png" width="150"></li>
-<h2> Week 2 </h2>
+</ul>
+<br>
+<li> Experiment 2 </li>
+<ul class="a">
+<li> PCR purification of <b> CcdB operon</b>: nanodrop
+<br>p5: 54.8 ng/µl
+<br>p10: 65.8 ng/µl
+<br>p20: 21.1 ng/µl</li>
+<li><b>cPCR</b> with Taq polymerase of colonies pSB6A1 (primers: MDM0096 and CLG0019) and pSB4A5 (primers: MDM0095 and CLG0019): <b>negative</b>
+<li> New <b>transformation</b> with pSB3T5, pSB4A5 and pSB6A1 using heat shock in <i>E. coli</i> <b>DH5a</b>
+<br> -> Plate on normal plates and glucose plates (100 ml 2% glucose, to avoid leaky expressing of <i>ccdB</i>)
+<br> -> Plates with transformants: pSB6A1 some colonies, pSB4A5 some colonies and pSB3T5 no colonies </li>
+<li>Gel elektroforesis on RD-fragments from plasmids: show expected fragments</li>
+<li><b>cPCR</b> on the pSB4A5 (primers: MDM0095 and CLG0019) and pSB6A1 (primers: MDM0096 and CLG0019) colonies with Taq polymerase: one <b>positive</b> colony of pSB6A1-T7<i>ccdB</i> (fragment of 437 bp in lane 14) <br>
+<img src="https://static.igem.org/mediawiki/2013/d/d8/UGent_2013_pSB6A1gel.jpg" width="200"/></a></li>
+<li><b>inoculation</b> of positive pSB6A1-T7<i>ccdB</i> colony from back up plate (3x: one for sequencing, 1 for cryovial and 1 for experiment 3)</li>
+<li>Plate <b>transformation mixtures</b> again on glucose plates and grow overnight at 30°C
+<br>->Plates with transformants: pSB4A5 colonies, pSB3T5 no colonies</li>
+<li><b>cPCR</b> on pSB4A5 colonies (primers: MDM0095 and CLG0019) with Taq polymerase: <b>negative</b></li>
+<li>New <b>ligation</b> with rest of RD-fragments of plasmids pSB3T5 (2 times) and pSB4A5 and CcdB from experiment 6 and <b>transformation</b> in DH5a using heat shock</li>
+<li>Due to lack of success: <b>start from the beginning</b>.</li>
+<li><b>Inoculation</b> of pSB3T5, pSB4A5, p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p10SpFRT-T7<i>ccdB</i> from cryovials.
+<br> <img src="https://static.igem.org/mediawiki/2013/e/ee/UGent_2013_plasmids_for_purification.png" width="200"/></a></li>
+<li>Also resuspend pSB3T5 (plate 5, well 7C) from iGEM kit, <b>transform</b> in <i>E. coli</i> DH5a using heat shock, plate on tetracycline plates and incubate overnight at 37°C
+<br> -> no colonies
+<br> -> transform again in DH5a using heat shock
+<br> -> again no colonies</li>
+<li>Purification of plasmids using Qiagen spin minikit: concentrations deduced from gel
+<br>p5SpFRT-T7<i>ccdB</i>: +/- 40 ng/µl
+<br>p10SpFRT-T7<i>ccdB</i>: +/- 40 ng/µl
+<br>p20SpFRT-T7<i>ccdB</i>: +/- 40 ng/µl
+<br>pSB3T4: +/- 250 ng/µl
+<br>pSB4A5 (1): +/- 400 ng/µl
+<br>pSB4A5 (2): +/- 350 ng/µl </li>
+<li>PCR on <b>CcdB operon</b> using Q5 polymerase (primers: MDM0586_Fw-Trc-<i>ccdB</i>-G00000 and MDM0587_Rv-Trc-<i>ccdB</i>-G00001) </li>
+<li><b>cPCR</b> on pSB3T5 colonies from old plates using Taq polymerase (primers: MDM0602 and CLG0019, expected fragment of 503 bp): <b>negative</b></li>
+<li><b>Restriction</b> of ccdB operon, pSB3T5 and pSB4A5 using PstI-HF and XbaI (gel purify RD-fragments using Qiagen Qiaquick gel extraction kit (expected fragment of 2157 bp for T7-<i>ccdB</i>, 3229 bp for pSB3T5 and 3372 bp for pSB4A5): concentrations deduced from gel</li>
+<li><b>Ligation</b> of pSB3T5 and T7-<i>ccdB</i> (from p5SpFRT-T7<i>ccdB</i>), pSB4A5 and T7-<i>ccdB</i> (from p5SpFRT-T7<i>ccdB</i>) and pSB4A5 and T7-<i>ccdB</i> (from p20SpFRT-T7<i>ccdB</i>) with T4 DNA ligase at 16°C overnight</li>
+<li><b>Transformation</b> of ligation mixtures in DH5a using heat shock
+<br>-> no colonies</li>
+</ul>
+<br>
+<li> Experiment 3 </li>
+<ul class="a">
+<li> Inoculation KI-strain 5 & 8 from experiment 1 </li>
+<li> <b> Transformation of pSB6A1 - T7-<i>ccdB</i> </b> in KI-strains 5 and 8 </li>
+<li> <b> Colony PCR </b>on kolonies from transformed strains using emerald polymerase with out primers to check KI: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> positive </b> </li>
+<li> <b> Colony PCR </b>on kolonies from transformed strains using emerald polymerase with MDM0096 & CLG0019 to check if plasmid is present. Expected fragment: 437 bp. Analytic gel: <b> positive </b><br>
+<img src="https://static.igem.org/mediawiki/2013/b/b7/UGent_2013_CPCR_KI%2Bplasmid.png" width="150"></li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li> New <b>transformation</b> in <i> E. coli </i> Top10 subcloning cells, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>negative</b>
+<li> <b>CcdB operon</b>: HiFi PCR of plasmids p20SpFRT-T7<i>ccdB</i> with MDM0586/MDM0587 to amplify CcdB operon</li>
+<li> New <b>restriction</b> of CcdB operon and pSB1C3 with Xba
+I and PstI
+<br> -> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br> Restriction Digest of T7-<i>ccdB</i>: 16.6 ng/µl
+<br> Restriction Digest of pSB1C3: 17.7 ng/µl</li>
+<li> <b>Ligation</b> of CcdB operon and pSB1C3: overnight at 16°C</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> -> Plate on chloramphenicol + glucose plate and grow overnight at 30°C: <b>negative</b>
+<li> <b>Restriction</b> of CcdB operon and pSB1C3 with XbaI and PstI
+<br> Because a preparative gel purification cause low concentrations, we will use DpnI
+<br> -> Purification by using minElute reaction cleanup kit</li>
+<li> Control of restriction fragments: <b>positive</b>, so we hope that ligation will succeed</li>
+<li> <b>Ligation</b> of CcdB operon and pSB1C3: overnight at 16°C</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>negative</b>
+<br> (it does not work, maby our transformation is not succeed)
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 4: august 19 - 25   {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 2 </li>
+<ul class="a">
+<li>pSB6A1-T7<i>ccdB</i> sent for sequencing with primers MDM0096 (A471969), MDM0060 (A471682) and MDM0039 (A471681)
+<br>-> <b>correct sequence</b></li>
+<li><b>Transform</b> ligation mixtures again in DH5a, using heat shock (42°C),
+<br>-> no colonies</li>
+<li><b>PCR on CcdB operon</b> with Q5 polymerase (primers: MDM0586_Fw-Trc-<i>ccdB</i>-G00000 & MDM0587_Rv-Trc-<i>ccdB</i>-G00001) and PCR purification using Qiagen Qiaquick PCR purification kit: nanodrop
+<br>p5: 15.2 ng/µl
+<br>p10: 18.6 ng/µl
+<br>p20: 43.5 ng/µl </li>
+<li>Inoculation of pSB3T5 and pSB4A5 from cryovials and plasmid purification using Qiagen Spin minikit: nanodrop
+<br>pSB3T5: 75.7 ng/µl
+<br>pSB4A5: 190.0 ng/µl </li>
+<li><b>Restriction</b> of CcdB operon, pSB3T5, pSB4A5 and the pSB6A1-T7<i>ccdB</i> transformant with PstI-HF and XbaI (gel purify restriction digest-fragments using Qiagen Qiaquick gel extraction kit (expected fragment of 2157 bp for T7-<i>ccdB</i>, 3229 bp for pSB3T5 and 3372 bp for pSB4A5)</li>
+<li><b>Ligation</b></li>
+<li><b>Transformation</b> in <i>E. coli</i> DH5a
+<br>-> no colonies
+<br>-> plate transformants on plates with a lower antibiotic concentration (50% lower)
+<br>-> no colonies</li>
+<li>Design primers for <b>Gibson assembly</b></li>
+</ul>
+<br>
+<li> Experiment 3 </li>
+<ul class="a">
+<li> <b> Colony PCR with higher annealing temperature to minimize false priming</b> on kolonies from transformed strains using emerald polymerase with out primers to check KI: MDM0046/MDM0010. Expected fragment: ca. 5500 bp. Analytic gel: <b> positive </b> </li>
+<li> <b> HiFi PCR using Q5 polymerase with two primer pairs generating overlapping fragments of the ccdA.gfp.cat construct </b>: MDM0046 (out) & MDM0123: 2130 bp and MEMO1237 & MDM0010 (out): 3400 bp. Analytic gel: <b>negative</b> </li>
+</ul>
+<br>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> <b> Lysate preparation</b>:<br>
+ -> Dilution of o/n culture of BW26547 in 5 mL LB+MgCL2+CaCl2+glucose <br>
+ -> Add phage lysate (10,20,40 & 80 µL)<br>
+ -> Wait untill lysis visible </li>
+<li> <b> Perform CIChE with 8 + pSB6A1 & 5 + pSB6A1 </b> (we will do 2 strains parallel): 0,0mM - 0,05mM IPTG </li>
+<li> <b> Transduction</b> of CIChe strains: no positive colonies after UV-test </li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li> New <b>transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> (because we are sure that the fragments were present for ligation and so will lead to succesful results)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>negative</b> (it still does not work) </li>
+<li> Control of ligations by using PCR with primers MDM0606 and MDM0607: <b>negative</b> </li>
+<li> <b>Ligation</b> again of CcdB operon and pSB1C3: 15 minutes at 16°C</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>negative</b> </li>
+<li> <b>CcdB operon</b>: HiFi PCR of plasmids p20SpFRT-T7<i>ccdB</i> with MDM0586/MDM0587 to amplify CcdB operon
+<br> because we have no more T7-<i>ccdB</i> fragments</li>
+<li> New <b>restriction</b> of CcdB operon and pSB1C3 with XbaI and PstI
+<br> -> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br> Restriction Digest of T7-<i>ccdB</i>: 15.3 ng/µl
+<br> Restriction Digest of pSB1C3: 16.8 ng/µl</li>
+<li> <b>Ligation</b> of CcdB operon and pSB1C3: 1 hour at room temperature</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>positive</b> (finally)</li>
+<li> <b>Colony PCR</b> (Taq): <b>negative</b>
+<br> It seems that restriction-ligation does not work, thus we will use another technique, called Gibson Assembly </li>
+<li> Designing primers for Gibson Assembly for the insert T7-<i>ccdB</i> and the backbone pSB1C3  </li>
+</ul>
+</ul>
+<br>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 5: august 26 - september 1   {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 2 </li>
+<ul class="a">
+<li> Inoculation of pSB3T5, pSB4A5, pSB6A1-T7<i>ccdB</i>, p5SpFRT-T7<i>ccdB</i>, p10pFRT-T7<i>ccdB</i> and p20pFRT-T7<i>ccdB</i> and plasmid purification using Qiagen Spin minikit: nanodrop
+<br>p10pFRT-T7<i>ccdB</i>: 62.8 ng/µl
+<br>p20pFRT-T7<i>ccdB</i>: 286.1 ng/µl</li>
+<li><b>PCR on CcdB operon</b> using Q5 polymerase (primers: MDM0586_Fw-Trc-<i>ccdB</i>-G00000 and MDM0587_Rv-Trc-<i>ccdB</i>-G00001): nanodrop
+<br>p10: 29.7 ng/µl
+<br>p20: 31.4 ng/µl</li>
+<li><b>Restriction</b> of pSB3T5, pSB4A5 and CcdB operon with PstI-HF and XbaI (gel purify RD-fragments using Qiagen Qiaquick gel extraction kit (expected fragment of 2157 bp for T7-<i>ccdB</i>, 3229 bp for pSB3T5 and 3372 bp for pSB4A5): nanodrop:
+<br>pSB3T5: 2.7 ng/µl
+<br>pSB4A5: 7.8 ng/µl
+<br> T7-<i>ccdB</i>: 10.5 ng/µl</li>
+<li> <b>Q5 PCR</b> of CcdB operon and plasmids (pSB3T5 and pSB4A5), using the designed Gibson primers
+<br> -> Purification of PCR-product after DpnI treatment by using minElute reaction cleanup kit
+<br> -> Control of fragments on a gel => Backbones are present, CcdB operons not </li>
+<li> <b>PrimeStar PCR</b> of CcdB operons, using the designed Gibson primers
+<br> -> Purification of PCR-product after DpnI treatment by using minElute reaction cleanup kit
+<br> -> Control of fragments on a gel => CcdB operons are still not present </li>
+<li> <b>Q5 PCR</b> of CcdB operons on a linear CcdB operon, using the designed Gibson primers
+<br> -> Purification of PCR-product, using Qiagen Qiaquick PCR purification kit,
+<br> -> Control of fragments on a gel => CcdB operon is visible </li>
+<li> <b>Gibson Assembly</b> (1h at 50°C)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C)
+<br> -> Plate pSB3T5 on tetracyclin plate and grow overnight at 37°C: <b>positive</b>
+<br> -> Plate pSB4A5 on ampicillin plate and grow overnight at 37°C:  <b>positive</b>
+<br> Strange phenomena: most colonies are red, let’s control it </li>
+<li> <b>Colony PCR</b> of colonies derived from Gibson Assembly: <b>negative</b>  </li>
+</ul>
+<br>
+<li> Experiment 3 </li>
+<ul class="a">
+<li> <b> Transformation </b> of plasmids:p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i>, p20SpFRT-T7<i>ccdB</i> in KI-strain (8) and back-up strain 5 </u> </li>
+<li><b>Colony PCR</b> on 5 + pSB6A1/p5/p10/p20 using emerald polymerase with primerpairs MDM0046/MDM010 to check KI. Expected fragment: 5500bp. Analytic gel: <b> positive </b> <br><img src="https://static.igem.org/mediawiki/2013/8/88/UGent_2013_CPCR_MDMcm.jpg" width="150"></li>
+<li><b>Colony PCR</b> on 5 + pSB6A1/p5/p10/p20 using emerald polymerase with primerpairs MDM0096/CGL0019 for pSB6A1 and MDM0039/MDM0060 for p5/p10/p20. Expected fragment: 437bp & 910 bp. Analytic gel: <b> positive for p5/p10/p20</b> </li>
+<li><b> New transformation </b> 5 +pSB6A1 and check KI + plasmid as described above. Analytic gel: <b> positive </b>.</li>
+</ul>
+<br>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> <b> Abort CIChe with 8+pSB6A1 & 5+pSB6A1 </b> because of mutation in pSB6A1 </li>
+<li> Lysate preparation </li>
+<li> <b> Transduction:  </b> on CIChE strains described above </li>
+<li> Test lysate by performing transduction on strain 5 with different concentrations of lysate: <b>negative</b> </li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li><b>While waiting for the Gibson Assembly primers  </b></li>
+<ul class="a">
+<li>  Again <b>restriction</b> of CcdB operon and pSB1C3 with XbaI and PstI
+<br> -> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br> Restriction Digest of T7-<i>ccdB</i>: 10.5 ng/µl
+<br> Restriction Digest of pSB1C3: 7.2 ng/µl</li>
+<li> <b>Ligation</b> of CcdB operon and pSB1C3: overnight at 16°C</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C),
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>positive</b>  </li>
+<li> <b>Colony PCR</b> (Taq) of these colonies: <b>negative</b>
+</ul>
+<li> <b>After receiving the primers for Gibson Assembly</b>
+<ul class="a">
+<li> <b>Q5 PCR</b> of CcdB operon and pSB1C3, using the designed Gibson primers
+<br> -> Purification of PCR-product, after DpnI treatment, by using minElute reaction cleanup kit
+<br> -> Control of fragments on a gel => Backbone is present, CcdB operon not </li>
+<li> <b>PrimeStar PCR</b> of CcdB operon, using the designed Gibson primers
+<br> -> Purification of PCR-product, after DpnI treatment, by using minElute reaction cleanup kit
+<br> -> Control of fragments on a gel => CcdB operon is not present </li>
+<li> <b>Q5 PCR</b> of CcdB operon on a linear CcdB operon, using the designed Gibson primers
+<br> -> Purification of PCR-product, using Qiagen Qiaquick PCR purification kit
+<br> -> Control of fragments on a gel => CcdB operon is visible </li>
+<li> <b>Gibson Assembly</b> (1h at 50°C)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C),
+<br> -> Plate on chloramphenicol plate and grow overnight at 37°C: <b>positive</b>
+<br> Strange phenomena: colonies are red, let’s control it </li>
+<li> <b>Colony PCR</b> (Taq) of colonies derived from Gibson Assembly: <b>negative</b>
+<br> We think that some of the original plasmid has to be present
+<br> and the bacteria love that plasmid more than the plasmid with T7-<i>ccdB</i></li>
+</ul>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}<html>
+<h2> September </h2>
+</html>{{:Team:UGent/Templates/ToggleBoxStart}}Week 1: september 2 - 8 {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 2 </li>
+<ul class="a">
+<li>  <b>Restriction</b> of CcdB operon and pSB3T5 with EcoRI and SpeI
+<br>-> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br>Restriction Digest of T7-<i>ccdB</i>: 14.4 ng/µl
+<br>Restriction Digest of pSB3T5 :  7.2 ng/µl
+<li>  <b>Restriction</b> of CcdB operon and pSB4A5 with EcoRI and SpeI
+<br>-> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br>Restriction Digest of T7-<i>ccdB</i>: 14.4 ng/µl
+<br>Restriction Digest of pSB4A5: 7.8 ng/µl
+<li> <b>Ligation</b> of CcdB operon and pSB3T5 and of CcdB operon and pSB4A5: 25 minutes at room temperature </li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a using heat shock
+<br> -> Plate pSB3T5 on tetracyclin plate and grow overnight at 37°C: <b>negative</b>
+<br> -> Plate pSB4A5 on ampicillin plate and grow overnight at 37°C: <b>negative</b> </li>
+<li> <b>Gibson Assembly</b> (1h at 50°C) of pSB3T5 and CcdB operon</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.3)
+<br>-> Plate on tetracyclin plate and grow overnight at 37°C: <b>negative</b> </li>
+<li> <b>Gibson Assembly</b> (1h at 50°C) of pSB4A5 and CcdB operon</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.4)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C:<b>negative</b> </li>
+</ul>
+<br>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> <b> CIChE with strain 8 + pSB6A1/p5/p10&p20:</b>
+<br> --> Inoculated without antibiotic & plated out on antibiotic: 0mM - 0.5mM IPTG
+<br> --> Inoculated in antibiotic - sequentially: 0mM - 0.5mM IPTG
+<br> --> Inoculated in antibiotic - parallel: 0mM -0.5 mM IPTG </li>
+<li> <b> Transduction: </b> on CIChE strains described above --> colonies on control plate </li>
+</ul>
+<br>
+<li> Experiment 5 </li>
+<ul class="a">
+<li> Test evaluation GFP with LB-medium:
+<br> -> Wild type
+<br> -> DH5a + pTGD-ccd-Pmb1GFP-CmFRT
+<br> -> Strains with GFP: 8 / 5 + pSB6A1/p5/p10/p20 -- 0mM & 0.01 mM IPTG </li>
+<li> Test evaluation GFP with EZrich-medium:
+<br> -> Wild type
+<br> -> DH5a + pTGD-ccd-Pmb1GFP-CmFRT
+<br> -> Strains with GFP: 8 / 5 + pSB6A1/p5/p10/p20 -- 0mM/0.01mM/0.05mM & 0.2mMM IPTG </li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li>  <b>Restriction</b> of CcdB operon and pSB1C3 with EcoRI and SpeI
+<br>-> Gel purify fragments using Qiagen Qiaquick gel extraction kit: nanodrop:
+<br>Restriction Digest T7-<i>ccdB</i>: 14.4 ng/µl
+<br>Restriction Digest pSB1C3: 4.4 ng/µl
+<li> <b>Ligation</b> of CcdB operon and pSB1C3: 25 minutes at room temperature </li>
+<li> <b>Transformation</b> in <i>E. coli</i> DH5a, using heat shock (42°C),
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C : <b>negative</b>  </li>
+<li> <b>Q5 PCR</b> of pSB1C3, using the designed Gibson primers and the linearised plasmid
+<br> -> Purification of PCR-product, using Qiagen Qiaquick PCR purification kit: nanodrop:
+<br> pSB1C3-backbone: 109.9 ng/µl</li>
+<li> <b>Gibson Assembly</b> (1h at 50°C)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.4)
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C: <b>positive</b> </li>
+<li> <b>Colony PCR</b> (Crimson) using primers MDM0606 and MDM0607:
+<br> 6 colonies can possible be <b>positive</b>  (but it is not sure)
+<br>-> Inoculate the 6 colonies (overnight)</li>
+<li>Control of fragment of pSB1C3 on a gel => Backbone is not present</li>
+<li>Plasmid purification of the 6 colonies + restriction to control of they are the good colonies (on a gel)
+<br> There is a possibility that they are the good ones, so we will send it to sequenate
+<br> -> pSB1C3-T7<i>ccdB</i> sent for <b>sequencing</b> with primers MDM0606, MDM0607, MDM0060 and MDM0039: <b>negative</b>  </li>
+<li> <b>Q5 PCR</b>  of pSB1C3, using the designed Gibson primers and the linearised plasmid
+<br>-> Purification of PCR-product, using Qiagen Qiaquick PCR purification kit:
+<br> nanodrop: pSB1C3-backbone: 58.0 ng/µl
+<br> -> Control of fragment of pSB1C3 on a gel => Backbone is not present</li>
+<li> <b>Q5 PCR</b>  of pSB1C3, using the designed Gibson primers and the restriction digest of pSB1C3
+<br>-> Purification of PCR-product, using Qiagen Qiaquick PCR purification kit:
+<br>nanodrop: pSB1C3-backbone: 76.2 ng/µl
+<br> -> Control of fragment of pSB1C3 on a gel => Backbone is present</li>
+<li> <b>Gibson Assembly</b> (1h at 50°C)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.3) </li>
+-> Plate on chloramphenicol plate and grow overnight at 37°C: <b>positive</b> => many colonies</li>
+<li> <b>Colony PCR</b> (Crimson):
+<br> We tested 48 colonies (using primers MDM0606 and MDM0607) and 4 colonies show the right fragment (2520 bp)
+<br> The first 24 colonies <img src=" https://static.igem.org/mediawiki/2013/1/13/UGent_2013_pSB1C3_cPCR_w1_septI.png
+" width="200"/></a>, and the second 24 colonies  <img src=" https://static.igem.org/mediawiki/2013/0/0d/UGent_2013_pSB1C3_cPCR_w1_septII.png
+" width="200"/></a>
+<br>-> Inoculate these 4 good colonies</li>
+<li> Plasmid purification of the 4 colonies, using Qiagen Qiaprep Spin minikit: nanodrop:
+<br>-> pSB1C3 strain 1:  94.2 ng/µl
+<br>-> pSB1C3 strain 2: 163.4 ng/µl
+<br>-> pSB1C3 strain 3: 160.2 ng/µl
+<br>-> pSB1C3 strain 4: 124.3 ng/µl</li>
+<li> <b>Restriction</b> with BspHI to control on a gel of they are the right colonies
+<br>(expected fragments are 1028bp and 3248 bp): <b>positive</b>
+<br>-> Strains 2, 3 and 4 seems to be the correct colonies</li>
+<li> pSB1C3-T7<i>ccdB</i> of these 3 colonies sent for <b>sequencing</b> with primers MDM0606, MDM0607, MDM0060 and MDM0039
+<br>-> sequence shows a mutation in the stop-codon, so we have to start over again</li>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 2: september 9 - 15 {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 2 </li>
+<ul class="a">
+<li> <b>Q5 PCR</b> for amplification of T7-<i>ccdB</i>-fragment, using the designed Gibson primers, on p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i>ccdB</i>
+<br> -> Using DpnI at 37°C for 1 hour
+<br> -> Purification of PCR-product by using minElute reaction cleanup kit
+<br> -> Control on gel: <b>negative</b>
+<li> Plasmid pSB3T5</li>
+<ul class="a">
+<li> <b>Gibson Assembly</b> (1h at 50°C) of pSB3T5 and CcdB operon that we already amplified before</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 3.0)
+<br>-> Plate on tetracyclin plate and grow overnight at 37°C: <b> negative</b>, there are oly red colonies</li>
+</ul>
+<li> Plasmid pSB4A5</li>
+<ul class="a">
+<li> <b>Gibson Assembly</b> (1h at 50°C) of pSB4A5 and CcdB operon that we already amplified before</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.0)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b>positive</b> </li>
+<li> <b>Colony PCR</b> (Crimson): there is only 1 colony. We tested this colony (using primers MDM0606 and MDM0607) and it show the right fragment (2486 bp) on gel
+<br><img src="https://static.igem.org/mediawiki/2013/3/31/UGent_2013_Ene_colonie_4A5.jpg"  width="50"/>
+<br>-> Inoculate these colonies</li>
+<li> Plasmid purification of the colonies, using Qiagen Qiaprep Spin minikit</li>
+<li> Seqenate this plasmid: the result is a totally different sequence than expected </li>
+</ul>
+<li> Plasmid pSB6A1</li>
+<ul class="a">
+<li> We controled the pSB6A1 on mutations (by sequencing) and we found also a mutation on in the <i>ccdB</i> gene</li>
+<li> Try to design Gibson primers to undo the mutations
+<br>(We will use primers to amplify the biggest part of the plasmid (PCR) and afterwards using Gibson Assembly with oligos, which undo the founded mutation) </li>
+<li> <b>Q5 PCR</b> for amplification of biggest part of the plasmid pSB6A1 (using the designed Gibson primers).
+<br> -> Using DpnI at 37°C for 1 hour
+<br> -> Purification of PCR-product by using minElute reaction cleanup kit
+<br> -> Control on gel: <b>positive</b> (fragment length is 6192bp)</li>
+<li> <b>Gibson Assembly</b>
+<br> -> melt oligos first: 5 minutes at 95°C
+<br> -> 6192bp-fragment and oligos at 50°C (1 h)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation  (Time Constant: 2.4)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b> positive</b> </li>
+<li> We made our own competent cells which have the <i>ccdA</i> gene in the genome, so they will be more tolerant to CcdB. We hope on no mutations this time.
+<br>-> <b>Q5 PCR</b>: Control of Knock-In
+<br> -> Control on gel: <b>positive</b>
+<br> <img src="https://static.igem.org/mediawiki/2013/0/08/UGent_2013_Control_ccda_competente_cellen.jpg"  width="50"/>
+<br> -> Further on we will call these cells competent strain 8
+</li>
+<li> Second <b>transformation</b> in competent strain 8, using electroporation  (Time Constant: 1.6)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b> negative</b> </li>
+<li> <b>Gibson Assembly</b>
+<br> -> melting oligos first: 5 minutes at 95°C + infinite at 50°C
+<br> -> 6192bp-fragment and oligos at 50°C (1 h)</li>
+<li> <b>Transformation</b> in competent strain 8, using electroporation (Time Constant: 1.7)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b> negative</b> </li>
+</ul>
+</ul>
+<br>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> CIChE with strain 8 + p5/p10/p20:
+<br> -> STEP: 0mM - 0.1mM IPTG
+<br> -> JUMP: 0mM - 0.5mM IPTG </li>
+<li> CIChE with strains 5 + p5/p10/p20:
+<br> -> STEP + JUMP: 0 - 0.01mM </li>
+</ul>
+<br>
+<li> Experiment 5 </li>
+<ul class="a">
+<li> <b> MTP experiment: version 1 (using precultures) </b>
+<br> (Evaluation GFP 4 colonies/strain -  3 repeats)
+<br> -> 8+pSB6A1 - sequential: 0mM - 0.5mM IPTG
+<br> -> 8+pSB6A1 - strains grown without antibiotics: 0mM - 0.5mM IPTG
+<br> -> 8+p10 - sequential: 0mM - 0.05mM  IPTG </li>
+<li> Measure the OD and the GFP (using FLUOstar)</li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li> <b>Q5 PCR</b> for amplification of T7-<i>ccdB</i>-fragment, using the designed Gibson primers, on p5SpFRT-T7<i>ccdB</i>, p10SpFRT-T7<i>ccdB</i> and p20SpFRT-T7<i>ccdB</i>
+<br> -> Using DpnI at 37°C for 1 hour
+<br> -> Purification of PCR-product by using minElute reaction cleanup kit
+<br> -> Control on gel: <b>negative</b>
+<li> <b>Gibson Assembly</b> (1h at 50°C), using a T7-<i>ccdB</i> we already amplified before</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation (Time Constant: 4.0)
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C: <b> negative</b> </li>
+<li> Try to design Gibson primers to undo the mutations, found in the <i>ccdB</i> gene
+<br>(We will use primers to amplify the biggest part of the plasmid (PCR) and afterwards using Gibson Assembly with oligos, which undo the founded mutation) </li>
+<li> <b>Q5 PCR</b> for amplification of biggest part of the plasmid (using the designed Gibson primers).
+<br> We will do this on the 2 best colonies of last time.
+<br> -> Using DpnI at 37°C for 1 hour
+<br> -> Purification of PCR-product by using minElute reaction cleanup kit
+<br> -> Control on gel: <b>positive</b> (fragment length is 4233bp)</li>
+<li> <b>Gibson Assembly</b>
+<br> -> melt oligos first: 5 minutes at 95°C
+<br> -> 4233bp-fragment and oligos at 50°C (1 h)</li>
+<li> <b>Transformation</b> in <i>E. coli</i> Top10 subcloning cells, using electroporation
+<br>(Time Constant for colony 1: 4.0, for colony 2: 4.1)
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C: <b> positive</b> </li>
+<li> We made our own competent cells which have the <i>ccdA</i> gene in the genome = strain 8, so they will be more tolerant to CcdB.
+<br> We hope on no mutations this time
+<br>-> <b>Q5 PCR</b>: Control of Knock-In
+<br> -> Control on gel: <b>positive</b>
+<br> <img src="https://static.igem.org/mediawiki/2013/0/08/UGent_2013_Control_ccda_competente_cellen.jpg"  width="50"/>
+</li>
+<li> Second <b>transformation</b> in competent strain 8, using electroporation
+<br>(Time Constant for colony 1: 1.5, for colony 2: 1.4)
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C: <b> positive</b> </li>
+<li> <b>Gibson Assembly</b>
+<br> -> melting oligos first: 5 minutes at 95°C + infinite at 50°C
+<br> -> 4233bp-fragment and oligos at 50°C (1 h)</li>
+<li> <b>Transformation</b> in competent strain 8, using electroporation (Time Constant for colony 1: 1.5, for colony 2: 1.4)
+<br>-> Plate on chloramphenicol plate and grow overnight at 37°C: <b> positive</b> </li>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 3: september 16 - 22 {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 2 </li>
+<ul class="a">
+<li> Plasmid pSB3T5</li>
+<ul class="a">
+<li> <b>Transformation</b> in competent strain 8, using electroporation  (Time Constant: 1.4)
+<br>-> Plate on tetracyclin plate and grow overnight at 37°C: <b> negative</b></li>
+<li> <b>Transformation</b> in competent strain 8, using electroporation
+<br> (Time Constant: pSB3T5+T7-<i>ccdB</i> of p10: 4.1,   pSB3T5+T7-<i>ccdB</i> of p20: 2.2)
+<br>-> Plate on tetracyclin plate and grow overnight at 37°C: <b> positive</b>, but also red colonies </li>
+<li> <b>Colony PCR</b> (Crimson):
+<br> We tested 15 colonies (using primers MDM0606 and MDM0607) : <b> negative</b> (expected fragment: 2486 bp)</li>
+</ul>
+<li> Plasmid pSB4A5</li>
+<ul class="a">
+<li> <b>Transformation</b> in competent strain 8, using electroporation  (Time Constant: 1.5)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b> negative</b></li>
+<li> <b>Transformation</b> in competent strain 8, using electroporation
+<br> (Time Constant: pSB3T5+T7-<i>ccdB</i> of p10: 2.7,  pSB3T5+T7-<i>ccdB</i> of p20: 2.6)
+<br>-> Plate on ampicillin plate and grow overnight at 37°C: <b> positive</b>, but also red colonies  </li>
+<li> <b>Colony PCR</b> (Crimson):
+ <br> We tested the few colonies, we had (using primers MDM0606 and MDM0607) : <b> negative</b> (expected fragment: 2486 bp)</li>
+</ul>
+<li> Plasmid pSB6A1</li>
+<ul class="a">
+<li> <b>Colony PCR</b> (Crimson):
+<br> We tested 24 colonies of pSB6A1(using primers MDM0606 and MDM0607) and  we found many good colonies
+<br> <img src=" https://static.igem.org/mediawiki/2013/9/9d/UGent_2013_pSB6A1_cPCR_w3_sept.png
+" width="200"/></a> (expected length is 4387 bp)
+<br>-> We chose 4 colonies to sequenate
+<br>->  Inoculate these 4 good colonies</li>
+<li> Plasmid purification of the 4 colonies, using Qiagen Qiaprep Spin minikit: nanodrop:
+<br>-> pSB6A1 strain 4 : 399.4 ng/µl
+<br>-> pSB6A1 strain 13: 412.0 ng/µl
+<br>-> pSB6A1 strain 16: 365.5 ng/µl
+<br>-> pSB6A1 strain 19: 420.3 ng/µl</li>
+<li> <b>Sequencing</b> shows in 2 colonies other mutations
+<br>and the other 2 colonies shows the right sequence
+<br>-> send this 2 good strains to iGEM (<b>BioBrick</b>)</li>
+</ul>
+</ul>
+<br>
+<li> Experiment 3 </li>
+<ul class="a">
+<li>Transformation
+</ul>
+<br>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> CIChE with strains 8 + p5/p10/p20:
+<br> -> STEP: 0.1mM - 1.0mM IPTG
+<br> -> JUMP: 0.5mM -  3mM IPTG </li>
+<li> CIChE with strains 5 + p5/p10/p20:
+<br> -> STEP: 0.01mM - 0.5mM IPTG
+<br> -> JUMP: 0.5mM - 1.0mM IPTG </li>
+<li> CIChE with strains 8 + pSB6A1 (New plasmids from colony 4 & 16 (exp 2)):
+<br> -> STEP: 0mM - 0.2mM IPTG
+<br> -> JUMP: 0.5mM - 5.0mM IPTG </li>
+</ul>
+<br>
+<li> Experiment 6 </li>
+<ul class="a">
+<li> <b>Colony PCR</b> (Crimson): We tested 24 colonies (using primers MDM0606 and MDM0607) and we found many good colonies
+<br> <img src=" https://static.igem.org/mediawiki/2013/2/25/UGent_2013_pSB1C3_cPCR_w3_sept.png
+" width="200"/></a> (expected length is 2520 bp)
+<br>-> We chose 4 colonies to sequenate
+<br>->  Inoculate these 4 good colonies</li>
+<li> Plasmid purification of the 4 colonies, using Qiagen Qiaprep Spin minikit: nanodrop:
+<br>-> pSB1C3 strain 10: 181.1 ng/µl
+<br>-> pSB1C3 strain 19: 169.1 ng/µl
+<br>-> pSB1C3 strain 20: 184.8 ng/µl
+<br>-> pSB1C3 strain 24: 184.5 ng/µl</li>
+<li> <b>Sequencing</b> shows the same mutation at the end codon again</li>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}{{:Team:UGent/Templates/ToggleBoxStart}}Week 4: september 23 - 29 {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> CIChE with strains 5 + p5/p10/P20:
+<br> -> STEP: 1.0mM - 4.0mM IPTG</li>
+<li> CIChE with strain 8 + pSB6A1:
+<br> -> STEP: 0.2mM - 2.0mM IPTG
+<br> -> JUMP: 5mM - 120mM IPTG</li>
+</ul>
+<br>
+<li> Experiment 5 </li>
+<ul class="a">
+<li> <b> MTP experiment: version 1 (using precultures) </b>
+<br> -> Plate1: 8 + p5;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate2: 8 + p10;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate3: 8 + p20;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate4: 8 + pSB6A1-16;STEP; 0mM Day1 - 0.05mM Day2
+<br> -> Plate5: 8 + p5;JUMP; 0mM Day1 - 2mM Day2
+<br> -> Plate6: 8 + p10;JUMP; 0mM Day1 - 2mM Day2
+<br> -> Plate7: 8 + p20;JUMP; 0mM Day1 - 2mM Day2
+</li>
+<li> Measure the OD and the GFP of all previous plates (using FLUOstar)</li>
+<li> <b> MTP experiment: Test version 2 </b>
+<br> (to know how long they have to grow until they reach a sufficient OD: 4 - 5 hours)
+</li>
+<li> <b> MTP experiment: version 2 </b>
+<br> -> Plate1: 8 + p5;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate2: 8 + p10;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate3: 8 + p20;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate4: 8 + pSB6A1-16;STEP; 0mM Day1 - 0.05mM Day2
+<br> -> Plate5: 8 + p5;JUMP; 0mM Day1 - 2mM Day2
+<br> -> Plate6: 8 + p10;JUMP; 0mM Day1 - 2mM Day2
+<br> -> Plate7: 8 + p20;JUMP; 0mM Day1 - 2mM Day2
+<br> -> Plate8: 8 + pSB6A1-16;STEP; 0.1mM Day1 - 0.2mM Day1 & JUMP;0mM Day1 - 5mM Day1
+<br> -> Plate9: 8 + pSB6A1-4;STEP; 0mM Day1 - 0.5mM Day2
+<br> -> Plate10: 8 + pSB6A1-4;STEP; 1.0mM Day1 - 2.0mM Day1 & JUMP; 0mM Day1 - 1.5mM Day1
+<br> -> Plate11: 8 + pSB6A1-4;JUMP; 1.5mM Day2 - 30.0mM Day2
+<br> -> Plate12: 8 + pSB6A1-4;JUMP; 60.0mM Day2 - 120.0mM Day1 <b>&</b> 5 + p5;STEP;0mM Day1 - 0.2mM Day1
+<br> -> Plate13: 5 + p5;STEP; 0.2mM Day2 - 3.0mM Day2
+<br> -> Plate14: 5 + p5;STEP; 3.5mM Day1 & JUMP;0mM Day1- 1mM Day1
+<br>    <b> & </b> 5 + p10;STEP;0mM Day1 - 0,01mM Day1
+<br> -> Plate15: 5 + p10;STEP; 0.01mM Day2 - 1.0mM Day2
+<br> -> Plate16: 5 + p10;STEP; 2mM Day1 - 3.5mM Day1 & JUMP;0mM Day1 - 0.1mM Day1
+<br> -> Plate17: 5 + p10;JUMP; 0.1mM Day2 - 1.0mM Day1 <b> & </b> 5 + p20;STEP; 0mM Day1 - 0.1mM Day2
+<br> -> Plate18: 5 + p20;STEP; 0.2mM Day1 - 3.0mM Day1
+<br> -> Plate19: 5 + p20;STEP; 3.0mM Day1 - 3.5mM Day1 & JUMP;0mM Day1 - 1mM day1
+</li>
+<li> Measure the OD and the GFP of all plates (using FLUOstar)</li>
+</ul
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}<html>
+<h2> October </h2>
+</html>{{:Team:UGent/Templates/ToggleBoxStart}}Week 1: september 30 - october 4 {{:Team:UGent/Templates/ToggleBoxStart1}}{{:Team:UGent/Templates/ToggleBoxStart2}}<html>
+<ul>
+<li> Experiment 4 </li>
+<ul class="a">
+<li> CIChE with strains 5 + p5/p10/P20:
+<br> -> STEP: 4.0mM - 5.0mM IPTG </li>
+<li> CIChE with strain 8 + pSB6A1:
+<br> -> STEP: 2.0mM - 3.0mM IPTG
+<br> -> JUMP: 120.0mM - 240mM IPTG</li>
+</ul>
+<br>
+<li> Experiment 5 </li>
+<ul class="a">
+<li> <b> MTP experiment: version 2 </b>
+<br> -> Plate20: 8 + pSB6A1-4;STEP; 2.5mM Day2 - 3.0mM Day2 & JUMP; 120mM Day2 - 240mM Day2
+<br> -> Plate21: 5 + p5;STEP; 3.5mM Day2 - 5mM Day2 <b>  &  </b> 5 + p10;STEP; 3.5mM Day2 - 5mM Day2
+<br> -> Plate22: 5 + p20;STEP; 3.5mM Day2 - 5mM Day2 <b>  &  </b> 5 + p5;STEP; 1mM Day1 and 3mM Day1
+<br><b>  &  </b> 5 + p10;STEP; 1mM Day1 and 3mM Day1<b>  &  </b> 5 + p20;STEP; 1mM Day1 and 3mM Day1
+</li>
+<li> Measure the OD and the GFP of the 3 plates (using FLUOstar)</li>
+</ul>
+</ul>
+</html>{{:Team:UGent/Templates/ToggleBoxEnd}}
-</html>
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Team:UGent/Labjournal

From 2013.igem.org

Latest revision as of 01:35, 5 October 2013

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