Team:Wageningen UR/notebook/journal/inhibition

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<h1>Fungal inhibition journal</h1>
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<h1>Fungal inhibition and greenhouse journal</h1>
                              
                              
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<h2 class="timelineMajorMarker"><span>May</span></h2>
<h2 class="timelineMajorMarker"><span>May</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
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<dt id="02w02"><a>Week 4</a></dt>
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<dt id="02w01"><a>Week 4</a></dt>
-
<dd class="timelineEvent" id="02w02EX" style="display:none;">
+
<dd class="timelineEvent" id="02w01EX" style="display:none;">
<p>Tranformed <i>E. coli</i> with BioBricks psb1C3, psb1A3, BBa_B0034. Grew transformants in 10 ml LB medium containing correct antibiotic and miniprepped them using a Genejet miniprep kit.
<p>Tranformed <i>E. coli</i> with BioBricks psb1C3, psb1A3, BBa_B0034. Grew transformants in 10 ml LB medium containing correct antibiotic and miniprepped them using a Genejet miniprep kit.
</p>
</p>
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<h2 class="timelineMajorMarker"><span>June</span></h2>
<h2 class="timelineMajorMarker"><span>June</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w03"><a>Week 1</a></dt>
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<dt id="02w02"><a>Week 1</a></dt>
-
<dd class="timelineEvent" id="02w03EX" style="display:none;">
+
<dd class="timelineEvent" id="02w02EX" style="display:none;">
<p>PCR methyl-γ-lyase with NEB  Q5 polymerase.  Used as templates: <br/> 1. Camembert cheese 2. <br/><i>Bevibacterium</i> strain isolated from sponge. Ran gel with 1 kb NEB ladder. Expected product size: 1.5 kbp.<br/>
<p>PCR methyl-γ-lyase with NEB  Q5 polymerase.  Used as templates: <br/> 1. Camembert cheese 2. <br/><i>Bevibacterium</i> strain isolated from sponge. Ran gel with 1 kb NEB ladder. Expected product size: 1.5 kbp.<br/>
Primers: <br/>
Primers: <br/>
Fw: 5’-GTTTCTTCGAATTCGCGGCCGCTTCTAGATGAGTATCACCCAGAACG-3'<br/>
Fw: 5’-GTTTCTTCGAATTCGCGGCCGCTTCTAGATGAGTATCACCCAGAACG-3'<br/>
Rev: 5’- GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATTCATACCGTTGCTACAGG-3'
Rev: 5’- GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATTCATACCGTTGCTACAGG-3'
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/c/c1/Wageningen_UR_notebook_wen_06_02_14_pcr_methyl-gamma-lyase.jpg/600px-Wageningen_UR_notebook_wen_06_02_14_pcr_methyl-gamma-lyase.jpg" width="400"><figcaption></figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/c/c1/Wageningen_UR_notebook_wen_06_02_14_pcr_methyl-gamma-lyase.jpg/600px-Wageningen_UR_notebook_wen_06_02_14_pcr_methyl-gamma-lyase.jpg" width="400"><figcaption>PCR methionine-gamma-lyase</figcaption></figure>
</p>
</p>
  </dd>
  </dd>
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<dl class="timelineMinor">
<dl class="timelineMinor">
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<dt id="02w04"><a>Week 2</a></dt>
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<dt id="02w03"><a>Week 2</a></dt>
-
<dd class="timelineEvent" id="02w04EX" style="display:none;">
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<dd class="timelineEvent" id="02w03EX" style="display:none;">
<p>Colony PCR with Q5 polymerase, using <i>P. putida</i> colonies as template. Ran gel with 100 bp NEB ladder. Expected bands size were around 500 bp.<br/>
<p>Colony PCR with Q5 polymerase, using <i>P. putida</i> colonies as template. Ran gel with 100 bp NEB ladder. Expected bands size were around 500 bp.<br/>
Primers:<br/>
Primers:<br/>
Fw: 5’-GTTTCTTCGAATTCGCGGCCGCTTCTAGATGGCGGAACAACTATCCACAAGTAAG<br/>
Fw: 5’-GTTTCTTCGAATTCGCGGCCGCTTCTAGATGGCGGAACAACTATCCACAAGTAAG<br/>
Rev: 5’- GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATCAGGCCTGGCGACTGGC<br/>  
Rev: 5’- GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATCAGGCCTGGCGACTGGC<br/>  
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/e/e6/Wageningen_UR_notebook_wen_06_10_14_pcr_pfri.jpg/600px-Wageningen_UR_notebook_wen_06_10_14_pcr_pfri.jpg" width="400"><figcaption>Extract pfrI from gel, digested it with SpeI and xbaI.  Ligated pfrI with BBa_B0034 (digested with SpeI).</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/e/e6/Wageningen_UR_notebook_wen_06_10_14_pcr_pfri.jpg/600px-Wageningen_UR_notebook_wen_06_10_14_pcr_pfri.jpg" width="400"><figcaption>PCR PfrI</figcaption></figure>
 +
<p>Extract pfrI from gel, digested it with SpeI and xbaI.  Ligated pfrI with BBa_B0034 (digested with SpeI).</p>
</p>
</p>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w05"><a>Week 3-4</a></dt>
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<dt id="02w04"><a>Week 3-4</a></dt>
-
<dd class="timelineEvent" id="02w05EX" style="display:none;">
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<dd class="timelineEvent" id="02w04EX" style="display:none;">
<p>Transformed chemical competent <i>E. coli</i> cells </p>
<p>Transformed chemical competent <i>E. coli</i> cells </p>
<ul>
<ul>
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<p>Psb1T3, psb1K3 transformants were grown in 10ml and then miniprepped.<br/>
<p>Psb1T3, psb1K3 transformants were grown in 10ml and then miniprepped.<br/>
Colony PCR with methyl-γ-lyase + BBa_B0034 transformant colonies using Taq polymerase. Primers were VF2 and a reverse primer from methyl-γ-lyase.  Ran gel with 1 kb NEB ladder. Is expect a band of around 1.5 kpb to appear if there was correct insertion of the product into the plasmid.<br/>
Colony PCR with methyl-γ-lyase + BBa_B0034 transformant colonies using Taq polymerase. Primers were VF2 and a reverse primer from methyl-γ-lyase.  Ran gel with 1 kb NEB ladder. Is expect a band of around 1.5 kpb to appear if there was correct insertion of the product into the plasmid.<br/>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/5/5a/Wageningen_UR_notebook_wen_06_16_14_colony_pcr_mgl.jpg/600px-Wageningen_UR_notebook_wen_06_16_14_colony_pcr_mgl.jpg" width="400"><figcaption>Sample 1, 2, 3 and 5 seem to have the correct insert. So glycerol stocks were made for sample 1 and 2.</figcaption></figure>
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<figure><img src="https://static.igem.org/mediawiki/2014/thumb/5/5a/Wageningen_UR_notebook_wen_06_16_14_colony_pcr_mgl.jpg/600px-Wageningen_UR_notebook_wen_06_16_14_colony_pcr_mgl.jpg" width="400"><figcaption>Colony PCR Methionine-gamma-lyase</figcaption></figure>
 +
Sample 1, 2, 3 and 5 seem to have the correct insert. So glycerol stocks were made for sample 1 and 2.
</p>
</p>
  </dd>
  </dd>
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<h2 class="timelineMajorMarker"><span>July</span></h2>
<h2 class="timelineMajorMarker"><span>July</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w06"><a>Week 1</a></dt>
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<dt id="02w05"><a>Week 1</a></dt>
-
<dd class="timelineEvent" id="02w06EX" style="display:none;">
+
<dd class="timelineEvent" id="02w05EX" style="display:none;">
<p>Sequencing data showed that Metionine-γ-lyase was inserted correctly together with Bba_b0034 (RBS), pfrI + B_0034 transformants were grown in 10 ml LB containing antibiotic and miniprepped. Plasmids were digested with EcoRI & SpeI. This was done because insert could enter in 2 ways, need to check for the correct insert.  Correct insert would give us 2132 bp and 566 bp, the incorrect insert will give us 5675 bp and 23 bp. Ran it with 1 kb NEB ladder.</p>
<p>Sequencing data showed that Metionine-γ-lyase was inserted correctly together with Bba_b0034 (RBS), pfrI + B_0034 transformants were grown in 10 ml LB containing antibiotic and miniprepped. Plasmids were digested with EcoRI & SpeI. This was done because insert could enter in 2 ways, need to check for the correct insert.  Correct insert would give us 2132 bp and 566 bp, the incorrect insert will give us 5675 bp and 23 bp. Ran it with 1 kb NEB ladder.</p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/1/14/Wageningen_UR_notebook_wen_06_30_14_schematic_drawing.jpg" width="300"><figcaption></figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/1/14/Wageningen_UR_notebook_wen_06_30_14_schematic_drawing.jpg" width="300"><figcaption>Schematic drawing of digestion and ligation strategy</figcaption></figure>
-
<figure><img src="https://static.igem.org/mediawiki/2014/b/b9/Wageningen_UR_notebook_wen_06_30_14_pfri_digest.jpg" width="400"><figcaption></figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/b/b9/Wageningen_UR_notebook_wen_06_30_14_pfri_digest.jpg" width="400"><figcaption>PfrI digest with EcoRI & SpeI</figcaption></figure>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w07"><a>Week 2</a></dt>
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<dt id="02w06"><a>Week 2</a></dt>
-
<dd class="timelineEvent" id="02w07EX" style="display:none;">
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<dd class="timelineEvent" id="02w06EX" style="display:none;">
-
<p>Grew <i>E. coli</i> containing SEVA plasmid 256, 581 and 434 in LB medium with correct antibiotic. Miniprepped them the day after.  Want to create SEVA plasmid that has pBBR1 ori, lacIq-Ptrc promoter and km or tet resistance. SEVA plasmids were digest with PacI and SpeI in order to get the cargo out, want to change the cargo and insert the correct cargo which is the lacIq-Ptrc (in SEVA 434) to backbones from 256 (Km resistant)0 and 581 (tet resistant). For SEVA 256 and 581 alkaline phosphatase was added in the digestion mixture. <br/></p>
+
<p>Grew <i>E. coli</i> containing SEVA plasmid 256, 581 and 434 in LB medium with correct antibiotic. Miniprepped them the day after.  Want to create SEVA plasmid that has pBBR1 ori, <i>lacIq-Ptrc</i> promoter and km or tet resistance. SEVA plasmids were digest with PacI and SpeI in order to get the cargo out, want to change the cargo and insert the correct cargo which is the lacIq-Ptrc (in SEVA 434) to backbones from 256 (Km resistant)0 and 581 (tet resistant). For SEVA 256 and 581 alkaline phosphatase was added in the digestion mixture. <br/></p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/2/25/Wageningen_UR_notebook_wen_06_07_14_SEVA_plasmid.jpg" width="200"><figcaption></figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/2/25/Wageningen_UR_notebook_wen_06_07_14_SEVA_plasmid.jpg" width="200"><figcaption>SEVA plasmid</figcaption></figure>
<p>
<p>
PCR was done with plasmid SEVA 434 using Q5 poly from NEB with primers:<br/>
PCR was done with plasmid SEVA 434 using Q5 poly from NEB with primers:<br/>
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Ran 5 μl of it through gel with a 1 kb plus GeneRuler ladder.
Ran 5 μl of it through gel with a 1 kb plus GeneRuler ladder.
<br/></p>
<br/></p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/a/a1/Wageningen_UR_notebook_wen_06_07_14_SEVA_434.jpg" width="300"><figcaption></figcaption></figure><p>
+
<figure><img src="https://static.igem.org/mediawiki/2014/a/a1/Wageningen_UR_notebook_wen_06_07_14_SEVA_434.jpg" width="300"><figcaption>lacIq-Ptrc PCR using SEVA 434 as template</figcaption></figure><p>
PCR purified rest of the PCR samples. Digested lacIq-Ptrc with PacI and SpeI then ligated with SEVA 581 (tet) and SEVA256 (km)  backbones. Did overnight ligation then afterwards ligase was deactivated by putting ligation mixture in 70°C for 10 min.  
PCR purified rest of the PCR samples. Digested lacIq-Ptrc with PacI and SpeI then ligated with SEVA 581 (tet) and SEVA256 (km)  backbones. Did overnight ligation then afterwards ligase was deactivated by putting ligation mixture in 70°C for 10 min.  
</p>
</p>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w03"><a>Week 3</a></dt>
+
<dt id="02w07"><a>Week 3</a></dt>
-
<dd class="timelineEvent" id="02w03EX" style="display:none;">
+
<dd class="timelineEvent" id="02w07EX" style="display:none;">
<p>PCR phlABCDE gene from <i>Psuedomonas protegens</i> pf-5 with Q5 polymerase and a tm of 63°C.<br/>
<p>PCR phlABCDE gene from <i>Psuedomonas protegens</i> pf-5 with Q5 polymerase and a tm of 63°C.<br/>
Primers are: <br/>
Primers are: <br/>
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<figure>
<figure>
<img src="https://static.igem.org/mediawiki/2014/0/05/Wageningen_UR_notebook_wen_07_22_gel_dapg.jpg">
<img src="https://static.igem.org/mediawiki/2014/0/05/Wageningen_UR_notebook_wen_07_22_gel_dapg.jpg">
-
<figcaption>Picture from DAPG</figcaption>
+
<figcaption>PCR <i>phl (DAPG)</i> gene cluster</figcaption>
</figure>
</figure>
<br/>
<br/>
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<figure>
<figure>
<img src="https://static.igem.org/mediawiki/2014/thumb/b/b1/Wageningen_UR_notebook_wen_07_22_SEVA_transformants_digest.jpg/472px-Wageningen_UR_notebook_wen_07_22_SEVA_transformants_digest.jpg">
<img src="https://static.igem.org/mediawiki/2014/thumb/b/b1/Wageningen_UR_notebook_wen_07_22_SEVA_transformants_digest.jpg/472px-Wageningen_UR_notebook_wen_07_22_SEVA_transformants_digest.jpg">
-
<figcaption>All transformants seemed to be correct, took #2 to be shuttle vector. Renamed it SEVA 254 which has a kanymcin resistance.</figcaption>
+
<figcaption>SEVA transformants digest.</figcaption>
</figure>
</figure>
 +
All transformants seemed to be correct, took #2 to be shuttle vector. Renamed it SEVA 254m contains a kanymcin resistance.
<p>
<p>
Digested the following:<br/>
Digested the following:<br/>
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<br/>
<br/>
<p>
<p>
-
Transformed in commercially competent <i>E. coli</i> cell using the ligations that were done above. </p>
+
Transformed in commercially competent <i>E. coli</i> cell using the ligations that were done above. <br/><br/>
 +
Chitinase sequence transformation to pSB1A3 into <i>E. coli</i> (unsuccesful attempt).</p>
                                                      
                                                      
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w03"><a>Week 4</a></dt>
+
<dt id="02w08"><a>Week 4</a></dt>
-
<dd class="timelineEvent" id="02w03EX" style="display:none;">
+
<dd class="timelineEvent" id="02w08EX" style="display:none;">
<p>Transformation of SEVA 254 containing genes was successful. Did a colony PCR for Methionine-γ-lyase and <i>PfrI</i> transformants. <br/><br/>
<p>Transformation of SEVA 254 containing genes was successful. Did a colony PCR for Methionine-γ-lyase and <i>PfrI</i> transformants. <br/><br/>
Using same primers that was used in order to amplify the gene. Used Taq polymerase with tm of 64°C. Ran PCR with a 2-log NEB ladder. Upper lane is Methionine-γ-lyase and lower lane is <i>PfrI</i>. Positive and negative control are indicated as + and – respectively. + control was for Methionine-γ-lyase <i>B. linens</i> and <i>PfrI</i> was <i>P. putida</i> KT2440.</p>  
Using same primers that was used in order to amplify the gene. Used Taq polymerase with tm of 64°C. Ran PCR with a 2-log NEB ladder. Upper lane is Methionine-γ-lyase and lower lane is <i>PfrI</i>. Positive and negative control are indicated as + and – respectively. + control was for Methionine-γ-lyase <i>B. linens</i> and <i>PfrI</i> was <i>P. putida</i> KT2440.</p>  
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/9/9a/Wageningen_UR_notebook_wen_pfri_colony_pcr.jpg/503px-Wageningen_UR_notebook_wen_pfri_colony_pcr.jpg"><figcaption></figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/9/9a/Wageningen_UR_notebook_wen_pfri_colony_pcr.jpg/503px-Wageningen_UR_notebook_wen_pfri_colony_pcr.jpg"><figcaption>pfri colony PCR</figcaption></figure>
<p>Made glycerol stocks for #4 and 5 of Methionine-γ-lyase and pfrI.
<p>Made glycerol stocks for #4 and 5 of Methionine-γ-lyase and pfrI.
Miniprepped and digest <i>phlABCDE</i> in SEVA 254 with xbaI and SpeI. If it cuts, then gene was inserted in the correct direction. Ran gel with 2-log NEB ladder.</p>
Miniprepped and digest <i>phlABCDE</i> in SEVA 254 with xbaI and SpeI. If it cuts, then gene was inserted in the correct direction. Ran gel with 2-log NEB ladder.</p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/2/20/Wageningen_UR_notebook_wen_07_21_seva254_dapg_dig.png/743px-Wageningen_UR_notebook_wen_07_21_seva254_dapg_dig.png"><figcaption>Took #2 and made glycerol stocks.</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/2/20/Wageningen_UR_notebook_wen_07_21_seva254_dapg_dig.png/743px-Wageningen_UR_notebook_wen_07_21_seva254_dapg_dig.png"><figcaption>SEVA254 DAPG digest</figcaption></figure>
 +
Took #2 and made glycerol stocks.
<p>
<p>
Transformed P.putida KT2440 using electroporation:</p>
Transformed P.putida KT2440 using electroporation:</p>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w06"><a>Week 5</a></dt>
+
<dt id="02w09"><a>Week 5</a></dt>
-
<dd class="timelineEvent" id="02w06EX" style="display:none;">
+
<dd class="timelineEvent" id="02w09EX" style="display:none;">
<p>Did colony PCR with <i>P. putida</i> transformants containing SEVA 254 <i>PfrI</i>. Ran PCR with 2-log NEB ladder. + control was a SEVA 254 <i>PfrI</i> plasmid.</p>
<p>Did colony PCR with <i>P. putida</i> transformants containing SEVA 254 <i>PfrI</i>. Ran PCR with 2-log NEB ladder. + control was a SEVA 254 <i>PfrI</i> plasmid.</p>
                                                     </dd>
                                                     </dd>
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<h2 class="timelineMajorMarker"><span>August</span></h2>
<h2 class="timelineMajorMarker"><span>August</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w05"><a>Week 1</a></dt>
+
<dt id="02w10"><a>Week 1</a></dt>
-
<dd class="timelineEvent" id="02w05EX" style="display:none;">
+
<dd class="timelineEvent" id="02w10EX" style="display:none;">
<p>Did colony PCR with <i>P. putida</i> transformants containing SEVA 254 <i>phlABCDE</i>. Ran PCR with 2-log NEB ladder. Positive control was a SEVA 254 <i>phlABCDE</i> plasmid. Used A the reverse primer of the gene a forward primer that it in the end gene where the product forms is around 1 kb. Annealing temperature used was: 52°C .These primes were chosen because we had troubles with colony PCR-ing >5kb. <br/><br/>
<p>Did colony PCR with <i>P. putida</i> transformants containing SEVA 254 <i>phlABCDE</i>. Ran PCR with 2-log NEB ladder. Positive control was a SEVA 254 <i>phlABCDE</i> plasmid. Used A the reverse primer of the gene a forward primer that it in the end gene where the product forms is around 1 kb. Annealing temperature used was: 52°C .These primes were chosen because we had troubles with colony PCR-ing >5kb. <br/><br/>
Primers used:<br/>
Primers used:<br/>
Fw: 5’-GTGCTGGTGACCTCGATTGC-3’<br/>
Fw: 5’-GTGCTGGTGACCTCGATTGC-3’<br/>
Rev:5’-GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTA CTAGTCCTTCAGGGGCAAG-3’</p>
Rev:5’-GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTA CTAGTCCTTCAGGGGCAAG-3’</p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f6/Wageningen_UR_notebook_wen_08_04_colonypcr_dapg.png/800px-Wageningen_UR_notebook_wen_08_04_colonypcr_dapg.png" width="400"><figcaption>Continued with number 6.</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f6/Wageningen_UR_notebook_wen_08_04_colonypcr_dapg.png/800px-Wageningen_UR_notebook_wen_08_04_colonypcr_dapg.png" width="400"><figcaption>Colony PCR DAPG</figcaption></figure>
 +
Continued with number 6.
 +
 
 +
<p>Chitinase sequence transformation to pSB1A3 into <i>E. coli</i> (unsuccesful attempt).
 +
Primers for colony PCR:<br/>
 +
FW: VF2 primer<br/>
 +
Rev:5'-AGGTGCTGCAGGAGCGTCATGGCTGA<br/>
 +
and<br/>
 +
FW: 5'GTGGATAAGATCGATTTTGCATCAA<br/>
 +
Rev:5'-AGGTGCTGCAGGAGCGTCATGGCTGA
 +
</p>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w06"><a>Week 2</a></dt>
+
<dt id="02w11"><a>Week 2</a></dt>
-
<dd class="timelineEvent" id="02w06EX" style="display:none;">
+
<dd class="timelineEvent" id="02w11EX" style="display:none;">
<p>Set up HPLC machine in order to detect 2,4-DAPG.  
<p>Set up HPLC machine in order to detect 2,4-DAPG.  
-
Ran 2,4-DAPG standard in HPLC.
+
Ran 2,4-DAPG standard in HPLC. ALso did a colony PCR with PfrI tranformants
</p>
</p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/e/e8/Wageningen_UR_notebook_wen_07_28_colony-pcr_pfri.png/800px-Wageningen_UR_notebook_wen_07_28_colony-pcr_pfri.png" width="400"><figcaption>Continued with number 3 and 4.</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/e/e8/Wageningen_UR_notebook_wen_07_28_colony-pcr_pfri.png/800px-Wageningen_UR_notebook_wen_07_28_colony-pcr_pfri.png" width="400"><figcaption>Colony PCR pfri</figcaption></figure>
 +
Continued with number 3 and 4.
                                                     </dd>
                                                     </dd>
</dl>
</dl>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w07"><a>Week 3</a></dt>
+
<dt id="02w12"><a>Week 3</a></dt>
-
<dd class="timelineEvent" id="02w07EX" style="display:none;">
+
<dd class="timelineEvent" id="02w12EX" style="display:none;">
<p>Synethetic methionine-γ-lyase arrived. Grew transformed plasmid to <i>E. coli</i>. Grew transformants and mini-prepped the day after.<br/>  
<p>Synethetic methionine-γ-lyase arrived. Grew transformed plasmid to <i>E. coli</i>. Grew transformants and mini-prepped the day after.<br/>  
Digested the following:</p>
Digested the following:</p>
<ul><li>SEVA 254 EcoRI & PstI</li>
<ul><li>SEVA 254 EcoRI & PstI</li>
<li>synthetic methionine-γ-lyase in IDT vector EcoRI & PstI</li></ul>
<li>synthetic methionine-γ-lyase in IDT vector EcoRI & PstI</li></ul>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f1/Wageningen_UR_notebook_wen_08_18_colonypcr_seva_mgl.png/453px-Wageningen_UR_notebook_wen_08_18_colonypcr_seva_mgl.png" width="200"><figcaption> Lower band of MgL and backbone band were gel extracted and then ligated together. Transformed in <i>E. coli</i>.  Ran a colony PCR (Taq pol) with the only transformant and ran gel with 2-log NEB ladder. + control was methionine-γ-lyase in IDT vector.</figcaption></figure> <br/>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f1/Wageningen_UR_notebook_wen_08_18_colonypcr_seva_mgl.png/453px-Wageningen_UR_notebook_wen_08_18_colonypcr_seva_mgl.png" width="200"><figcaption>Colony PCR SEVA Methionine-gamma-lyase(MgL)</figcaption></figure>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/d/d3/Wageningen_UR_notebook_wen_08_18_dig_seva_mgl.png/550px-Wageningen_UR_notebook_wen_08_18_dig_seva_mgl.png" width="200"><figcaption> Transformant is correct, grew it in liq LB, mini-prepped day after. Transformed in <i>P. putida</i> KT2440. </figcaption></figure>
+
Lower band of MgL and backbone band were gel extracted and then ligated together. Transformed in <i>E. coli</i>.  Ran a colony PCR (Taq pol) with the only transformant and ran gel with 2-log NEB ladder. + control was methionine-γ-lyase in IDT vector.
 +
<br/>
 +
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/d/d3/Wageningen_UR_notebook_wen_08_18_dig_seva_mgl.png/550px-Wageningen_UR_notebook_wen_08_18_dig_seva_mgl.png" width="200"><figcaption>Digest SEVA MgL</figcaption></figure>
 +
Transformant is correct, grew it in liq LB, mini-prepped day after. Transformed in <i>P. putida</i> KT2440.
 +
 
 +
<p>Chitinase transformation into <i>P. putida</i> in pSEVA254 (succesfully). <br/>
 +
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/1/18/Wageningen_UR_chitinase_tjasa1.png/778px-Wageningen_UR_chitinase_tjasa1.png" width="300" height="350"><figcaption>SnapGene scheme</figcaption></figure><br/><br/>
 +
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/5/5f/Wageningen_UR_chit_in_seva_putida_white.jpg/600px-Wageningen_UR_chit_in_seva_putida_white.jpg" width="400"><figcaption>PCR colony of <i>P. putida</i>. Expected bands were ~750 bp which were prooved by sequencing.</figcaption></figure>
                                                     </dd>
                                                     </dd>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w08"><a>Week 4</a></dt>
+
<dt id="02w13"><a>Week 4</a></dt>
-
<dd class="timelineEvent" id="02w08EX" style="display:none;">
+
<dd class="timelineEvent" id="02w13EX" style="display:none;">
-
<p>Did Pyoverdine growth experiments (see protocols).</p>
+
<p>Did Pyoverdine growth experiments (see protocols).
 +
</p>
                                                     </dd>
                                                     </dd>
</dl>
</dl>
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<h2 class="timelineMajorMarker"><span>September</span></h2>
<h2 class="timelineMajorMarker"><span>September</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w09"><a>Week 1</a></dt>
+
<dt id="02w14"><a>Week 1</a></dt>
-
<dd class="timelineEvent" id="02w09EX" style="display:none;">
+
<dd class="timelineEvent" id="02w14EX" style="display:none;">
 +
<h3>Greenhouse</h3>
 +
<p>Banana plants were transfered to soil.
 +
</p>
 +
<br/>
 +
<h3>Fungal inhibition</h3>
<p>Did a growth experiment with <i>phl P. putida</i> transformants (contains <i>phl</i> gene cluster in order to produce 2,4-DAPG) in 100ml medium in 1L erlenmeyer flasks.  Done in duplo’s.</p>
<p>Did a growth experiment with <i>phl P. putida</i> transformants (contains <i>phl</i> gene cluster in order to produce 2,4-DAPG) in 100ml medium in 1L erlenmeyer flasks.  Done in duplo’s.</p>
<ul><li>WT <i>P. putida</i> KT2440</li>
<ul><li>WT <i>P. putida</i> KT2440</li>
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Digested synthetic Methionine-γ-lyase in IDT best fit and psb1C3 vector with EcoRI and PstI. Purified digestion and ligated overnight. <br/>
Digested synthetic Methionine-γ-lyase in IDT best fit and psb1C3 vector with EcoRI and PstI. Purified digestion and ligated overnight. <br/>
Transformed plasmids <i>Pfri</i> (psb1C3) and Methionine-γ-lyase (psb1C3) to <i>E. coli</i> DH5-α commercial competent cells.<br/>  
Transformed plasmids <i>Pfri</i> (psb1C3) and Methionine-γ-lyase (psb1C3) to <i>E. coli</i> DH5-α commercial competent cells.<br/>  
-
Also transformed SEVA 254 containing synthetic Methionine-γ-lyase to <i>P. putida</i> KT2440.</p>
+
Also transformed SEVA 254 containing synthetic Methionine-γ-lyase to <i>P. putida</i> KT2440.<br/><br/>
 +
 
 +
Chitinase sequence transformation to pSB1A3 into <i>E. coli</i> (unsuccesful attempt).</p>  
 +
 
                                                     </dd>
                                                     </dd>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w11"><a>Week 2</a></dt>
+
<dt id="02w15"><a>Week 2</a></dt>
-
<dd class="timelineEvent" id="02w11EX" style="display:none;">
+
<dd class="timelineEvent" id="02w15EX" style="display:none;">
<p>Ran a colony PCR with <i>E. coli</i> transforamants with <i>PfrI</i> (psb1C3) and methionine-γ-lyase (psb1C3). Ran gel with 2-log NEB ladder. </p><br/>
<p>Ran a colony PCR with <i>E. coli</i> transforamants with <i>PfrI</i> (psb1C3) and methionine-γ-lyase (psb1C3). Ran gel with 2-log NEB ladder. </p><br/>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f0/Wageningen_UR_notebook_wen_09_08_1_mgl_pfri_colony_pcr.png/727px-Wageningen_UR_notebook_wen_09_08_1_mgl_pfri_colony_pcr.png" width="400"><figcaption>Upper lane is from methionine-γ-lyase (psb1C3) and lower lane is <i>PfrI</i> (psb1C3). Expected around 1.5kb for methionine-γ-lyase and around 600bp for <i>PfrI</i>. Numbers 1 and 2 were continued with both methionine-γ-lyase (psb1C3) and <i>PfrI</i> (psb1C3).</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/f/f0/Wageningen_UR_notebook_wen_09_08_1_mgl_pfri_colony_pcr.png/727px-Wageningen_UR_notebook_wen_09_08_1_mgl_pfri_colony_pcr.png" width="400"><figcaption>Mgl, PfrI colony PCR</figcaption></figure>
 +
Upper lane is from methionine-γ-lyase (psb1C3) and lower lane is <i>PfrI</i> (psb1C3). Expected around 1.5kb for methionine-γ-lyase and around 600bp for <i>PfrI</i>. Numbers 1 and 2 were continued with both methionine-γ-lyase (psb1C3) and <i>PfrI</i> (psb1C3).
<br/>
<br/>
<p>Grew and miniprepped these transformants. methionine-γ-lyase (psb1C3) plasmids were digested with EcoRI and PstI. Ran gel with 2-log NEB ladder. Expected a 1.5kb band (insert) with a 2.2 kb backbone.</p><br/>
<p>Grew and miniprepped these transformants. methionine-γ-lyase (psb1C3) plasmids were digested with EcoRI and PstI. Ran gel with 2-log NEB ladder. Expected a 1.5kb band (insert) with a 2.2 kb backbone.</p><br/>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/d/db/Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png/312px-Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png" width="200"><figcaption>Both plasmids are correct with 1.5kb insert band and a 2.2kb backbone, 3-4kb band are uncut plasmids.</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/d/db/Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png/312px-Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png" width="200"><figcaption>MgL EcoRI and PstI digestion</figcaption></figure>
 +
Both plasmids are correct with 1.5kb insert band and a 2.2kb backbone, 3-4kb band are uncut plasmids.
<p>Also did a mutagenesis with <i>PfrI</i> (psb1C3) plasmid with Q5 polymerase using primers: <br/>
<p>Also did a mutagenesis with <i>PfrI</i> (psb1C3) plasmid with Q5 polymerase using primers: <br/>
Line 282: Line 316:
Afterwards ran a gel for the mutagenesis. </p>
Afterwards ran a gel for the mutagenesis. </p>
-
<figure><img src="https://static.igem.org/mediawiki/2014/thumb/d/db/Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png/312px-Wageningen_UR_notebook_wen_09_08_2_mgl_dig.png" width="200"><figcaption>Both plasmids are correct with 1.5kb insert band and a 2.2kb backbone, 3-4kb band are uncut plasmids.</figcaption></figure>
+
<figure><img src="https://static.igem.org/mediawiki/2014/6/67/Wageningen_UR_notebook_wen_09_08_3_mutagenesis.png" width="200"><figcaption>mutagenesis</figcaption></figure>
 +
Both plasmids are correct with 1.5kb insert band and a 2.2kb backbone, 3-4kb band are uncut plasmids.
<p>Mutagenesis was succesfull with expected band size of 2.8kb and nothing on negative control. Afterwards added DpnI to purified mutagenesis plasmid and transformed into <i>E. coli</i> competent cells. <br/>
<p>Mutagenesis was succesfull with expected band size of 2.8kb and nothing on negative control. Afterwards added DpnI to purified mutagenesis plasmid and transformed into <i>E. coli</i> competent cells. <br/>
Line 299: Line 334:
<li><i>E. coli</i> with <i>phl</i> gene</li></ul>  
<li><i>E. coli</i> with <i>phl</i> gene</li></ul>  
-
<p>Grew them all for 48 hours before harvesting the agar plates. </p>
+
<p>Grew them all for 48 hours before harvesting the agar plates.<br/><br/>
 +
 
 +
Directed mutagenesis of Chitinase in pSEVA254 performed 3 times with different annealing temperatures (60°C, 50°C and 70°C) and different times of elongation (30 seconds per kb - 50 seconds per kb). None of them worked.</p>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w12"><a>Week 3</a></dt>
+
<dt id="02w16"><a>Week 3</a></dt>
-
<dd class="timelineEvent" id="02w12EX" style="display:none;">
+
<dd class="timelineEvent" id="02w16EX" style="display:none;">
 +
<h3>Greenhouse</h3>
 +
<p>Banana plants were transfered to bigger pots.
 +
</p>
 +
<br/>
 +
<h3>Fungal inhibition</h3>
<p>Cut agar in little pieces and extracted first with acetone and then with ethyl acetate. Prepared all HPLC samples and ran them in HPLC. Check <a href=" https://static.igem.org/mediawiki/2014/0/07/Wageningen_UR_protocols_DAPGprotocols.pdf " class="soft_link">protocols</a> for more details.</p>
<p>Cut agar in little pieces and extracted first with acetone and then with ethyl acetate. Prepared all HPLC samples and ran them in HPLC. Check <a href=" https://static.igem.org/mediawiki/2014/0/07/Wageningen_UR_protocols_DAPGprotocols.pdf " class="soft_link">protocols</a> for more details.</p>
<br/>
<br/>
Line 327: Line 369:
</ul>
</ul>
 +
<p>Chitinase sequence transformation to pSB1C3 into <i>E. coli</i> (unsuccesful attempt).</p>
                                                     </dd>
                                                     </dd>
</dl>
</dl>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w12"><a>Week 4</a></dt>
+
<dt id="02w17"><a>Week 4</a></dt>
-
<dd class="timelineEvent" id="02w12EX" style="display:none;">
+
<dd class="timelineEvent" id="02w17EX" style="display:none;">
<p>Plated 2,4-DAPG and DMDS on komada plates with concentrations being and inoculated <i>Fusarium</i> TR4 on these plates. Also co-inoculated <i>P. putida</i> and <i>Fusarium (foc)</i>.<br/>
<p>Plated 2,4-DAPG and DMDS on komada plates with concentrations being and inoculated <i>Fusarium</i> TR4 on these plates. Also co-inoculated <i>P. putida</i> and <i>Fusarium (foc)</i>.<br/>
Line 346: Line 389:
<h2 class="timelineMajorMarker"><span>October</span></h2>
<h2 class="timelineMajorMarker"><span>October</span></h2>
<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w13"><a>Week 1</a></dt>
+
<dt id="02w18"><a>Week 1</a></dt>
-
<dd class="timelineEvent" id="02w13EX" style="display:none;">
+
<dd class="timelineEvent" id="02w18EX" style="display:none;">
 +
<h3>Greenhouse</h3>
 +
<p>Banana plants were inoculated with 5 ml (OD600 of 0.25) of Pseudomonas putida expressing fungal growth inhibitors.
 +
2 days later banana plants were inoculated with 5 ml (1 mio spores per ml) of Fusarium and 2 inoculated maize kernels per plant.
 +
</p>
 +
<br/>
 +
<h3>Fungal inhibition</h3>
<p>Did a pyoverdine growth experiment. And also co-inoculated <i>P. putida</i> with <i>Fusarium</i> on agar plates for in vivo assay.</p>
<p>Did a pyoverdine growth experiment. And also co-inoculated <i>P. putida</i> with <i>Fusarium</i> on agar plates for in vivo assay.</p>
                                                     </dd>
                                                     </dd>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w14"><a>Week 2</a></dt>
+
<dt id="02w19"><a>Week 2</a></dt>
-
<dd class="timelineEvent" id="02w14EX" style="display:none;">
+
<dd class="timelineEvent" id="02w19EX" style="display:none;">
<p>Plated 2,4-DAPG and DMDS on komada plates with concentrations being and inoculated <i>Fusarium</i> TR4 on these plates. Also co-inoculated <i>P. putida</i> and <i>Fusarium (foc)</i>.
<p>Plated 2,4-DAPG and DMDS on komada plates with concentrations being and inoculated <i>Fusarium</i> TR4 on these plates. Also co-inoculated <i>P. putida</i> and <i>Fusarium (foc)</i>.
-
Did a pyoverdine growth experiment.</p>
+
Did a pyoverdine growth experiment.<br/>
 +
Performed a Chitinase growth experiment in <i>P. putida</i>.</p>
                                                     </dd>
                                                     </dd>
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<dl class="timelineMinor">
<dl class="timelineMinor">
-
<dt id="02w15"><a>Week 3</a></dt>
+
<dt id="02w20"><a>Week 3</a></dt>
-
<dd class="timelineEvent" id="02w15EX" style="display:none;">
+
<dd class="timelineEvent" id="02w20EX" style="display:none;">
<p>In co-inoculated more <i>Fusarium</i> with <i>P. putida</i>  on agar plates. Prepared inoculum for green house experiments. Inoculated them in the morning with overnight cultures, induced them at OD ~0.5, harvest after 4 hours and afterwards dilute them with LB medium to an OD of 0.25.<br/>
<p>In co-inoculated more <i>Fusarium</i> with <i>P. putida</i>  on agar plates. Prepared inoculum for green house experiments. Inoculated them in the morning with overnight cultures, induced them at OD ~0.5, harvest after 4 hours and afterwards dilute them with LB medium to an OD of 0.25.<br/>
Did a colony PCR with methionine-γ-lyase <i>P. putida</i> transformants, these were done with primers:<br/>  
Did a colony PCR with methionine-γ-lyase <i>P. putida</i> transformants, these were done with primers:<br/>  
Line 370: Line 420:
Rev: 5’- GGTCAGCGATAGGCACCTC-3’<br/>
Rev: 5’- GGTCAGCGATAGGCACCTC-3’<br/>
-
Found out that tranformants used for enzyme isolation in previous growth experiments were correct.</p>
+
Found out that tranformants used for enzyme isolation in previous growth experiments were correct.
 +
</p>
                                                     </dd>
                                                     </dd>
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Latest revision as of 03:47, 18 October 2014

Wageningen UR iGEM 2014

 

 

Fungal inhibition and greenhouse journal


May

Week 4

June

Week 1
Week 2
Week 3-4

July

Week 1
Week 2
Week 3
Week 4
Week 5

August

Week 1
Week 2
Week 3
Week 4

September

Week 1
Week 2
Week 3
Week 4

October

Week 1
Week 2
Week 3