Team:Cooper Union/Notebook/Telomere July

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<ul class="menu">
<ul class="menu">
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/TdT_project">De Novo Synthesis </a></li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/TdT_project">De Novo Synthesis </a></li>
-
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Telomere_project">Programmable Lifespan</a> </li>
+
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Telomere_project">Programmable Lifespan Timer</a> </li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Biohack_project">Biohacker Kit </a></li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Biohack_project">Biohacker Kit </a></li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Hardware">OpenSource Hardware </a> </li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Hardware">OpenSource Hardware </a> </li>
 +
<!--<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Modeling">Modeling </a> </li>-->
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Parts">BioBrick Parts </a></li>
<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Parts">BioBrick Parts </a></li>
-
<!--<li class="menu"> <a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Modeling">Modeling </a> </li>-->
 
</ul>
</ul>
</li>
</li>
-
<li class="menu-safety"> <a class="menu" href="https://igem.org/Safety/Safety_Form?team_id=1354">Safety</a> </li>
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<li class="menu-safety"> Social
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<li class="menu-outreach"><a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Outreach">Outreach </a></li>
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<ul class="menu">
 +
<li class="menu"><a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Safety">Safety</a> </li>
 +
<li class="menu"><a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Ethics">Ethics</a> </li>
 +
<li class="menu"><a class="menu" href="https://2014.igem.org/Team:Cooper_Union/Outreach">Outreach </a></li>
 +
</ul>
 +
</li>
<li class="menu-notebook">  Notebook  
<li class="menu-notebook">  Notebook  
<ul class="menu">
<ul class="menu">
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<div class="notebook-header">     
<div class="notebook-header">     
     <div class="left-side">
     <div class="left-side">
-
         <h1>Programmable Lifespan</h1>
+
         <h1>Programmable Lifespan Timer</h1>
     </div>
     </div>
     <div class="notebook-nav-container">
     <div class="notebook-nav-container">
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<img src=" https://static.igem.org/mediawiki/2014/3/31/CU_701_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/3/31/CU_701_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/1/14/CU_701_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/1/14/CU_701_1300.jpg " width="200" />
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<img src=" https://2014.igem.org/File:CU_701_W303alpha.jpg " width="200" />
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<img src=" https://static.igem.org/mediawiki/2014/8/87/CU_701_W303alpha.jpg" width="200" />
<br>
<br>
For tomorrow: run gel of PCR samples<br>
For tomorrow: run gel of PCR samples<br>
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<ul>
<ul>
<li>restreaked yeast plates from last week (the ones that were likely to be TRP);<br>
<li>restreaked yeast plates from last week (the ones that were likely to be TRP);<br>
-
     6 Plates restreaked at day 4 after day 1 (faint): W303alpha+TRP1-1, W303alpha negative control,          W303alpha+TRP1-3</li>
+
     6 Plates restreaked at day 4 after day 1 (faint): W303&alpha;+TRP1-1, W303&alpha; negative control,          W303&alpha;+TRP1-3</li>
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<li>Photos of yeast plates/restreaked: 1300, 1294, 1296,1297, w303alpha<br>
+
<li>Photos of yeast plates/restreaked: 1300, 1294, 1296,1297, w303&alpha;<br>
     Due to deletion of EST2, 1294,1296,1297 are fading:dying</li>
     Due to deletion of EST2, 1294,1296,1297 are fading:dying</li>
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<li>New transformation done by prof. Medvedik: wrong plates on original transformation</li>
<li>New transformation done by prof. Medvedik: wrong plates on original transformation</li>
-
<li>Ran gel with yesterday's PCR samples (MT, ML, VT, VL) with one of the De Novo group's pet28+TdT samples.  Used VersaLadder.  <br>Wells: 1. blank ; 2. ladder ; 3. VT ; 4. VL ; 5. MT ; 6. ML ; 7. pET28+TdT<br>
+
<li>Ran gel with yesterday's PCR samples (MT, ML, VT, VL) with one of the De Novo group's pet28+TdT samples.  Used VersaLadder.  <br><br><img src=" https://static.igem.org/mediawiki/2014/5/5a/CU_702_Gel_run.JPG " width="350" /><br>Wells: 1. blank ; 2. ladder ; 3. VT ; 4. VL ; 5. MT ; 6. ML ; 7. pET28+TdT<br><br>
<dl><dd>Sizes expected: 1074 for VT and MT, 2415 VL and ML</dd><dl></li>
<dl><dd>Sizes expected: 1074 for VT and MT, 2415 VL and ML</dd><dl></li>
<li>Results: we had to stain the gel with ethidium bromide because everything was too faint at first.<br>
<li>Results: we had to stain the gel with ethidium bromide because everything was too faint at first.<br>
  VL and ML had approximately 2kb; VT and MT had approximately 1kb --> good results! <br>
  VL and ML had approximately 2kb; VT and MT had approximately 1kb --> good results! <br>
-
However, there were other bands that showed along with the PCR amplification -- maybe raise temperature to 56 instead of 54.</li></ul>
+
However, there were other bands that showed along with the PCR amplification -- maybe raise temperature to 56&deg;C instead of 54&deg;C.</li></ul>
<br>
<br>
<img src=" https://static.igem.org/mediawiki/2014/a/ab/CU_702_1294.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/a/ab/CU_702_1294.jpg " width="200" />
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<img src=" https://static.igem.org/mediawiki/2014/c/cd/CU_702_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/c/cd/CU_702_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/8/84/CU_702_W303alpha.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/8/84/CU_702_W303alpha.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/5/5a/CU_702_Gel_run.JPG " width="200" />
 
<br>
<br>
For tomorrow:  run PCR with same samples, but with different temperature<br>
For tomorrow:  run PCR with same samples, but with different temperature<br>
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PCR machine not available, unable to do PCR<br>
PCR machine not available, unable to do PCR<br>
-
Restreaked cultures and took photoes<br>
+
Restreaked cultures and took photos<br>
Restreaked successful transformation colonies: Mak31+TRP1/VPS75+TRP1<br>
Restreaked successful transformation colonies: Mak31+TRP1/VPS75+TRP1<br>
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PCR: EST1+TRP1, EST1+LEU2<br>
PCR: EST1+TRP1, EST1+LEU2<br>
-
Culture preps: W303A, W303alpha, 1300, 1296<br>
+
Culture preps: W303A, W303&alpha;, 1300, 1296<br>
New YPD plates made<br>
New YPD plates made<br>
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Plates struck<br>
Plates struck<br>
-
Gel Run with 1% gel and 1k ladder: Two showed nothing while the third ET showed multiple bands.<br>
+
Gel Run with 1% gel and 1k ladder:<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/4/4e/CU_707_gel_run.jpg " width="350" /><br>
 +
Two showed nothing while the third ET showed multiple bands.<br><br>
-
Could be contamination in sample/annealing temperature problem (54->56, maybe try 58) <br>
+
Could be contamination in sample/annealing temperature problem (54&deg;C->56&degC, maybe try 58&deg;C) <br>
<br><br>
<br><br>
<img src=" https://static.igem.org/mediawiki/2014/b/bb/CU_707_1294.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/b/bb/CU_707_1294.jpg " width="200" />
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<img src=" https://static.igem.org/mediawiki/2014/5/56/CU_707_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/5/56/CU_707_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/1/1e/CU_707_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/1/1e/CU_707_1300.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/8/8a/CU_707_w303alpha.jpg " width="200" />
+
<img src=" https://static.igem.org/mediawiki/2014/8/8a/CU_707_w303alpha.jpg " width="200" /><br>
-
<img src=" https://static.igem.org/mediawiki/2014/4/4e/CU_707_gel_run.jpg " width="200" /><br>
+
<br>
-
 
+
Tomorrow: Transformation<br>
Tomorrow: Transformation<br>
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<h3>7/8/14</h3><em>(Nolana)</em>
<h3>7/8/14</h3><em>(Nolana)</em>
<ul>
<ul>
-
<li>Ran 1% gel of PCR samples ET1, ET2, EL1, ET2.  Wells: 2. BioLabs 1kb ladder ; 3. EL1 ; 3. EL2 ; ET1 ; ET2</li>
+
<li>Ran 1% gel of PCR samples ET1, ET2, EL1, ET2.  <br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/6/6b/CU_708_gel.jpg " width="350" />
 +
Wells: 2. BioLabs 1kb ladder ; 3. EL1 ; 3. EL2 ; ET1 ; ET2</li>
<li>Gel results were faint, so we stained the gel in ethidium bromide for 15 minutes. <br>
<li>Gel results were faint, so we stained the gel in ethidium bromide for 15 minutes. <br>
<dl><dt> Expected sizes -- ET: 1074 ; EL: 2415.</dt>
<dl><dt> Expected sizes -- ET: 1074 ; EL: 2415.</dt>
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<dd> miniprep LEU2 plasmid again?</dd></li>
<dd> miniprep LEU2 plasmid again?</dd></li>
<li>Checked and restreaked yeast plates to check for growth</li>
<li>Checked and restreaked yeast plates to check for growth</li>
-
<li>Yeast transformation of W303alpha, W303a, 1300, 1296</li>
+
<li>Yeast transformation of W303&alpha;, W303a, 1300, 1296</li>
<li>1296 discarded for transformation</li>
<li>1296 discarded for transformation</li>
<li>Knockout of EST1+TRP1/LEU2 for other strains in progress</li></ul>
<li>Knockout of EST1+TRP1/LEU2 for other strains in progress</li></ul>
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<img src=" https://static.igem.org/mediawiki/2014/7/72/CU_708_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/7/72/CU_708_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/3/39/CU_708_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/3/39/CU_708_1300.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/8/86/CU_708_W303alpha.jpg " width="200" />
+
<img src=" https://static.igem.org/mediawiki/2014/8/86/CU_708_W303alpha.jpg " width="200" /><br>
-
<img src=" https://static.igem.org/mediawiki/2014/6/6b/CU_708_gel.jpg " width="200" />
+
<br>
<br>
For tomorrow: Miniprep TRP, LEU<br>
For tomorrow: Miniprep TRP, LEU<br>
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<img src=" https://static.igem.org/mediawiki/2014/2/24/CU_709_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/2/24/CU_709_1297.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/7/78/CU_709_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/7/78/CU_709_1300.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/b/b1/CU_709_W303alpha.jpg " width="200" />
+
<img src=" https://static.igem.org/mediawiki/2014/b/b1/CU_709_W303alpha.jpg " width="200" /><br>
<br>
<br>
For tomorrow: re-miniprep plasmids for pFA6a-TRP1, pFA6a-LEU3MX6;<br>
For tomorrow: re-miniprep plasmids for pFA6a-TRP1, pFA6a-LEU3MX6;<br>
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<li>Miniprepped pFA6a-TRP1 and pFA6a-LEU2MX6 plasmid templates</li>
<li>Miniprepped pFA6a-TRP1 and pFA6a-LEU2MX6 plasmid templates</li>
<li><dl><dt>Nanodropped miniprep samples:</dt>
<li><dl><dt>Nanodropped miniprep samples:</dt>
-
<dd>TRP1: 298.4 ng/uL</dd>
+
<dd>TRP1: 298.4 ng/&mu;L</dd>
-
<dd>LEU2: 163.8 ng/uL</dd></dl></li>
+
<dd>LEU2: 163.8 ng/&mu;L</dd></dl></li>
<li>Yeast plates were restruck and photos were taken for growth monitoring</li>
<li>Yeast plates were restruck and photos were taken for growth monitoring</li>
<li>PCR'ed two samples each of EST1+LEU2, EST1+TRP1 for PCR purification and then yeast transformation tomorrow.<br>
<li>PCR'ed two samples each of EST1+LEU2, EST1+TRP1 for PCR purification and then yeast transformation tomorrow.<br>
-
PCR conditions:  program 333, temperature 54, 180 seconds extension time, 30 cycles</li>
+
PCR conditions:  program 333, temperature 54&deg;C, 180 seconds extension time, 30 cycles</li>
<li>Ran two 1% gels of yesterday's PCR product: <br>
<li>Ran two 1% gels of yesterday's PCR product: <br>
<dl><dd>gel 1 wells: 1-3: blank ; 4. MT1 ; 5: ML1 ; 6. VT1 ; 7. VL1 ; 8. Biolabs 100bp ladder</dd>
<dl><dd>gel 1 wells: 1-3: blank ; 4. MT1 ; 5: ML1 ; 6. VT1 ; 7. VL1 ; 8. Biolabs 100bp ladder</dd>
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PCR purification results: near 0 concentration: Redo PCR on Sunday<br>
PCR purification results: near 0 concentration: Redo PCR on Sunday<br>
-
Gels ran again<br>
+
Gels ran again<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/9/98/CU_711_Gel_1.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/9/94/CU_711_Gel_2.jpg " width="350" />
<dl><dd>gel 1 wells: 1blank ; 2. ladder 3. MT1 ; 4: ML1 ; 5. VT1 ; 6. VL1 </dd>
<dl><dd>gel 1 wells: 1blank ; 2. ladder 3. MT1 ; 4: ML1 ; 5. VT1 ; 6. VL1 </dd>
<dd>gel 2 wells: 1blank ; 2. Ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2 </dd></dl>
<dd>gel 2 wells: 1blank ; 2. Ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2 </dd></dl>
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<img src=" https://static.igem.org/mediawiki/2014/6/65/CU_711_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/6/65/CU_711_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/b/b2/CU_711_W303alpha.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/b/b2/CU_711_W303alpha.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/9/98/CU_711_Gel_1.jpg " width="200" />
+
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/9/94/CU_711_Gel_2.jpg " width="200" /><br>
+
For Monday: Tranformation, PCR purification<br>
For Monday: Tranformation, PCR purification<br>
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Overnight cultures of 1300. W303a. W303A remade<br>
Overnight cultures of 1300. W303a. W303A remade<br>
-
Gel run<br>
+
Gel run<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/d/d1/CU_714_Gel_run_gel_1.jpg " width="350" /><br>
<dl><dd>gel 1 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML1 ; 5. VT1 ; 6. VL1; 7 versa ladder</dd>
<dl><dd>gel 1 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML1 ; 5. VT1 ; 6. VL1; 7 versa ladder</dd>
<dd>gel 2 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2  ; 7.versa ladder</dd></dl>
<dd>gel 2 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2  ; 7.versa ladder</dd></dl>
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<img src=" https://static.igem.org/mediawiki/2014/3/39/CU_714_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/3/39/CU_714_1300.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/8/86/CU_714_W303a.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/8/86/CU_714_W303a.jpg " width="200" />
-
<img src=" https://static.igem.org/mediawiki/2014/d/d1/CU_714_Gel_run_gel_1.jpg " width="200" /><br>
+
<br>
Tomorrow: Check PCR (Gel/ purification), Transformation of 1300, W303a, W303A if PCR is successful.<br>
Tomorrow: Check PCR (Gel/ purification), Transformation of 1300, W303a, W303A if PCR is successful.<br>
<br>
<br>
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<h3>7/15/14</h3>
<h3>7/15/14</h3>
<ul>
<ul>
-
<li>Checked gel pictures from last gel run --</li>
+
<li>Checked gel pictures from last gel run<br>
-
<li>
+
<dl><dt>Expected sizes of gene w/out knockout:</dt>
<dl><dt>Expected sizes of gene w/out knockout:</dt>
<dd>MAK31: 381 bp</dd>
<dd>MAK31: 381 bp</dd>
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<dd>VPS75: 275 bp</dd></dl></li>
<dd>VPS75: 275 bp</dd></dl></li>
<li>Ran PCR of MT, ML, VT, VL (one regular, one universal sample) on the new OpenPCR machine, program 334:
<li>Ran PCR of MT, ML, VT, VL (one regular, one universal sample) on the new OpenPCR machine, program 334:
-
<dl><dd>Initial Step: Temp 95, Time 300</dd>
+
<dl><dd>Initial Step: Temp 95&deg;C, Time 300</dd>
-
<dd>Anneal: Temp 56, Time 30</dd>
+
<dd>Anneal: Temp 56&deg;C, Time 30</dd>
-
<dd>Extend: Temp 72, Time 30</dd>
+
<dd>Extend: Temp 72&deg;C, Time 30</dd>
-
<dd>Final Step: Temp 72, Time 420</dd>
+
<dd>Final Step: Temp 72&deg;C, Time 420</dd>
-
<dd>Final Hold: Temp 4</dd>
+
<dd>Final Hold: Temp 4&deg;C</dd>
<dd>Cycles: 30</dd></dl></li>
<dd>Cycles: 30</dd></dl></li>
-
<li>Ran two 1% gels (10uL PCR product, 2 uL 10x loading dye)<br>
+
<li>Ran two 1% gels (10uL PCR product, 2 uL 10x loading dye)<br><br>
 +
<img src="https://static.igem.org/mediawiki/2014/7/74/CU_715_Gel_1.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/9/9d/CU_715_Gel_2.jpg " width="350" /><br>
<dl><dd>Gel 1 wells: 1. blank ; 2. 100bp ladder ; 3. MT1 ; 4. ML1 ; 5. VT1 ; 6. VL1</dd>
<dl><dd>Gel 1 wells: 1. blank ; 2. 100bp ladder ; 3. MT1 ; 4. ML1 ; 5. VT1 ; 6. VL1</dd>
<dd>Gel 2 wells: 1. blank ; 2. 100bp ladder ; 3. MT2 ; 4. ML2 ; 5. VT2 ; 6. VL2</dd></dl>
<dd>Gel 2 wells: 1. blank ; 2. 100bp ladder ; 3. MT2 ; 4. ML2 ; 5. VT2 ; 6. VL2</dd></dl>
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<li>Ran PCR again with same settings, but with new colonies</li></ul>
<li>Ran PCR again with same settings, but with new colonies</li></ul>
<br>
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/7/74/CU_715_Gel_1.jpg " width="200" />
+
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/9/9d/CU_715_Gel_2.jpg " width="200" /><br>
+
For tomorrow: run gel<br>
For tomorrow: run gel<br>
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<dd>Colony 4: E-G</dd></dl></li>
<dd>Colony 4: E-G</dd></dl></li>
<li>Ran gels of all PCR samples for genes without knockouts (samples A-H)
<li>Ran gels of all PCR samples for genes without knockouts (samples A-H)
 +
<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/7/72/CU_716_Gel_ABCD1.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/8/82/CU_716_Gel_EFGH1.jpg " width="350" /><br>
<dl><dt>Gel run</dt>
<dl><dt>Gel run</dt>
<dd>gel 1.1 wells: 1blank ; 2. 250 base ladder ; 3. (A1) MT1 ; 4: (B1) ML1 ; 5. (C1) VT1 ; 6. (D1) VL1</dd>
<dd>gel 1.1 wells: 1blank ; 2. 250 base ladder ; 3. (A1) MT1 ; 4: (B1) ML1 ; 5. (C1) VT1 ; 6. (D1) VL1</dd>
<dd>gel 1.2 wells: 1blank ; 2. 250 base ladder ; 3. (E1) MT2 ; 4: (F1) ML2 ; 5. (G1) VT2 ; 6. (H1) VL2</dd></dl></li>
<dd>gel 1.2 wells: 1blank ; 2. 250 base ladder ; 3. (E1) MT2 ; 4: (F1) ML2 ; 5. (G1) VT2 ; 6. (H1) VL2</dd></dl></li>
-
<li>Ran gels of all PCR samples for genes with universal primers (samples A-H)<br>
+
<li>Ran gels of all PCR samples for genes with universal primers (samples A-H)<br><br>
 +
<br><img src=" https://static.igem.org/mediawiki/2014/6/6d/CU_716_Gel_ABCD_2.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/0/0e/CU_716_Gel_EFGH_2.jpg " width="350" /><br>
<dl><dt>Gel run</dt>
<dl><dt>Gel run</dt>
<dd>gel 2.1 wells: 1blank ; 2. 250 base ladder 3. (A2) MT1 ; 4: (B2) ML1 ; 5. (C2) VT1 ; 6. (D2) VL1</dd>
<dd>gel 2.1 wells: 1blank ; 2. 250 base ladder 3. (A2) MT1 ; 4: (B2) ML1 ; 5. (C2) VT1 ; 6. (D2) VL1</dd>
Line 319: Line 332:
<dd>gel 2.1 had one very bright VT band -- streak out this colony to double check later?</dd></dl></li></ul>
<dd>gel 2.1 had one very bright VT band -- streak out this colony to double check later?</dd></dl></li></ul>
<br>
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/6/6d/CU_716_Gel_ABCD_2.jpg " width="200" />
+
 
-
<img src=" https://static.igem.org/mediawiki/2014/7/72/CU_716_Gel_ABCD1.jpg " width="200" />
+
-
<img src=" https://static.igem.org/mediawiki/2014/0/0e/CU_716_Gel_EFGH_2.jpg " width="200" />
+
-
<img src=" https://static.igem.org/mediawiki/2014/8/82/CU_716_Gel_EFGH1.jpg " width="200" /><br>
+
For tomorrow:  screen more colonies!  If gels still show no deletions, then maybe do yeast transformation on Friday.<br>
For tomorrow:  screen more colonies!  If gels still show no deletions, then maybe do yeast transformation on Friday.<br>
Line 332: Line 342:
<dl><dd>Colony 5: A-D</dd>
<dl><dd>Colony 5: A-D</dd>
<dd>Colony 6: E-H</dd></dl></li>
<dd>Colony 6: E-H</dd></dl></li>
-
<li>Ran gels of all PCR samples for genes without knockouts (A-H 3)</li>
+
<li>Ran gels of all PCR samples for genes without knockouts (A-H 3)<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/0/0f/CU_717_Gel_ABCD3.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/2/2f/CU0717_Gel_EFGH3.jpg " width="350" /><br>
<dl><dt>Gel run</dt>
<dl><dt>Gel run</dt>
<dd>gel 1 wells: 1blank ; 2. 250 base ladder ; 3. (A3) MT1 ; 4: (B3) ML1 ; 5. (C3) VT1 ; 6. (D3) VL1</dd>
<dd>gel 1 wells: 1blank ; 2. 250 base ladder ; 3. (A3) MT1 ; 4: (B3) ML1 ; 5. (C3) VT1 ; 6. (D3) VL1</dd>
<dd>gel 2 wells: 1blank ; 2. 250 base ladder ; 3. (E3) MT2 ; 4: (F3) ML2 ; 5. (G3) VT2 ; 6. (H3) VL2</dd></dl></li>
<dd>gel 2 wells: 1blank ; 2. 250 base ladder ; 3. (E3) MT2 ; 4: (F3) ML2 ; 5. (G3) VT2 ; 6. (H3) VL2</dd></dl></li>
-
<li>Ran gels of all PCR samples for genes with universal primers (samples A-H 4)
+
<li>Ran gels of all PCR samples for genes with universal primers (samples A-H 4)<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/5/56/CU_717_Gel_ABCD4.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/3/35/CU_717_Gel_EFGH4.jpg " width="350" />
<dl><dt>Gel run</dt>
<dl><dt>Gel run</dt>
<dd>gel 3 wells: 1blank ; 2. 250 base ladder 3. (A4) MT1 ; 4: (B4) ML1 ; 5. (C4) VT1 ; 6. (D4) VL1</dd>
<dd>gel 3 wells: 1blank ; 2. 250 base ladder 3. (A4) MT1 ; 4: (B4) ML1 ; 5. (C4) VT1 ; 6. (D4) VL1</dd>
Line 344: Line 358:
<li>Restreaked VPS75:: TRP1 of colonies 3, 5, and 6</li></ul>
<li>Restreaked VPS75:: TRP1 of colonies 3, 5, and 6</li></ul>
<br>
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/0/0f/CU_717_Gel_ABCD3.jpg " width="200" />
 
-
<img src=" https://static.igem.org/mediawiki/2014/5/56/CU_717_Gel_ABCD4.jpg " width="200" />
 
-
<img src=" https://static.igem.org/mediawiki/2014/3/35/CU_717_Gel_EFGH4.jpg " width="200" />
 
-
<img src=" https://static.igem.org/mediawiki/2014/2/2f/CU0717_Gel_EFGH3.jpg " width="200" /><br>
 
For tomorrow: screen more colonies! MAK31 colonies<br>
For tomorrow: screen more colonies! MAK31 colonies<br>
Check restreaked colonies<br>
Check restreaked colonies<br>
Line 356: Line 366:
<ul>
<ul>
<li>Colony PCR'ed MAK31::TRP1 deletion strain. 10 samples: 5 samples from Plate A (A7-A11), 5 samples from Plate B (B1-B5).<br>PCR settings: program 334, anneal temp: 56, extension time: 30 sec.</li>
<li>Colony PCR'ed MAK31::TRP1 deletion strain. 10 samples: 5 samples from Plate A (A7-A11), 5 samples from Plate B (B1-B5).<br>PCR settings: program 334, anneal temp: 56, extension time: 30 sec.</li>
-
<li>Made two 1% agarose gels</li>
+
<li>Made two 1% agarose gels<br><br>
-
<li><dl><dt>Ran gels</dt>
+
<img src=" https://static.igem.org/mediawiki/2014/7/78/CU_718_Gel_1_Run_Plate_A.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/5/5c/CU_718_Gel_2_Run_Plate_B.jpg " width="350" /><br>
 +
<dl><dt>Ran gels</dt>
<dd>gel 1 wells: 1. blank ; 2. Versa ladder ; 3-6. A7-10 ; 7-8. Shoshana and Devora's samples</dd>
<dd>gel 1 wells: 1. blank ; 2. Versa ladder ; 3-6. A7-10 ; 7-8. Shoshana and Devora's samples</dd>
<dd>gel 2 wells: 1 blank ; 2. Versa ladder ; 3-7. B1-5 ; 8. A11</dd></dl></li>
<dd>gel 2 wells: 1 blank ; 2. Versa ladder ; 3-7. B1-5 ; 8. A11</dd></dl></li>
-
<li>Results: gel 1 had one faint band at A7, we stained the gel in 400 mL H2O and 500 uL ethidium bromide for 15 minutes. <br>
+
<li>Results: gel 1 had one faint band at A7, we stained the gel in 400 mL H<sub>2</sub>O and 500&mu;L ethidium bromide for 15 minutes. <br>
  After staining, the band was still faint.  All the Plate B samples on gel 2 had successful knockouts, but we realized the samples were taken from one streaked out colony.</li>
  After staining, the band was still faint.  All the Plate B samples on gel 2 had successful knockouts, but we realized the samples were taken from one streaked out colony.</li>
<li>Streaked out 2 YPD plates for the MAK31:TRP1 deletion: 1 plate B colony, A7</li>
<li>Streaked out 2 YPD plates for the MAK31:TRP1 deletion: 1 plate B colony, A7</li>
<li>Overnight PCR of Plate B colony to double-check deletion: one sample with universal primer, one sample with gene check primer</li></ul>
<li>Overnight PCR of Plate B colony to double-check deletion: one sample with universal primer, one sample with gene check primer</li></ul>
<br>
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/7/78/CU_718_Gel_1_Run_Plate_A.jpg " width="200" />
 
-
<img src=" https://static.igem.org/mediawiki/2014/5/5c/CU_718_Gel_2_Run_Plate_B.jpg " width="200" /><br>
 
For Monday: check the MAK31 colonies and the VPS colonies that were struck yesterday.<br>
For Monday: check the MAK31 colonies and the VPS colonies that were struck yesterday.<br>
Prepare for new transformations for those strains with EST1.<br>
Prepare for new transformations for those strains with EST1.<br>
Line 375: Line 385:
<li>Made four 1% agarose gels</li>
<li>Made four 1% agarose gels</li>
<li>ran PCR of VT colonies with possible knockouts that were streaked out last week.  6 samples: 2 of each colony (one with universal primer, one with gene check primer): colonies 3, 5, 6 using the OpenPCR program 334.</li>
<li>ran PCR of VT colonies with possible knockouts that were streaked out last week.  6 samples: 2 of each colony (one with universal primer, one with gene check primer): colonies 3, 5, 6 using the OpenPCR program 334.</li>
-
<li>Ran gel of last week's MT samples: 2 samples: one with universal primer, one with gene check primer. Wells: 1. blank ; 2. Versa ladder ; 3. universal ; 4. gene check</li>
+
<li>Ran gel of last week's MT samples: 2 samples: one with universal primer, one with gene check primer.<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/2/2e/CU_721_MT_gel.jpg " width="350" /><br>
 +
  Wells: 1. blank ; 2. Versa ladder ; 3. universal ; 4. gene check</li>
<li>Results: there were bands for both lanes on the gel, which corresponded to their respective sequence sizes (universal: 275, gene check: 406) -- maybe yeast strain is diploid?</li>
<li>Results: there were bands for both lanes on the gel, which corresponded to their respective sequence sizes (universal: 275, gene check: 406) -- maybe yeast strain is diploid?</li>
-
<li>Ran gel of VT colonies. Wells: 1. Versa ladder ; 2. 3R ; 3. 5R ; 4. 6R ; 5. 3U ; 6. 5U ; 7. 6U</li>
+
<li>Ran gel of VT colonies.<br><br>
-
<li>Results: bands were faint, stained gel in 200mL H2O+250uL ethidium bromide.  After staining, confirmed that 2 colonies had knockouts (3 and 6)</li>
+
<img src=" https://static.igem.org/mediawiki/2014/8/83/CU_721_VT_gel.jpg " width="350" /><br>
-
<li>Streaked out three plates of previous W303alpha transformation</li>
+
  Wells: 1. Versa ladder ; 2. 3R ; 3. 5R ; 4. 6R ; 5. 3U ; 6. 5U ; 7. 6U</li>
-
<li>Streaked out original 1808 colony (pre-transformation)</li></ul>
+
<li>Results: bands were faint, stained gel in 200mL H<sub>2</sub>O+250&mu;L ethidium bromide.  After staining, confirmed that 2 colonies had knockouts (3 and 6)</li>
 +
<li>Streaked out three plates of previous W303&alpha; transformation</li>
 +
<li>Streaked out original 1808 colony (pre-transformation)</li></ul><br>
<br>
<br>
-
<img src=" https://static.igem.org/mediawiki/2014/f/f6/CU_721_Gel_Run_Yeast.jpg " width="200" />
+
<img src=" https://static.igem.org/mediawiki/2014/f/f6/CU_721_Gel_Run_Yeast.jpg " width="350" />
-
<img src=" https://static.igem.org/mediawiki/2014/2/2e/CU_721_MT_gel.jpg " width="200" />
+
-
<img src=" https://static.igem.org/mediawiki/2014/8/83/CU_721_VT_gel.jpg " width="200" /><br>
+
For tomorrow: make more YPD plates, check MAK31 plates again, prepare for yeast transformation<br>
For tomorrow: make more YPD plates, check MAK31 plates again, prepare for yeast transformation<br>
Line 394: Line 406:
<li>Ran overnight PCR samples of EST1+LEU2 for tomorrow (purification and yeast transformation<br>
<li>Ran overnight PCR samples of EST1+LEU2 for tomorrow (purification and yeast transformation<br>
<dl><dt>Program: PCR for ~1-2kb 54c</dt>
<dl><dt>Program: PCR for ~1-2kb 54c</dt>
-
<dd>Initial Step: Temp 95, Time 300</dd>
+
<dd>Initial Step: Temp 95&deg;C, Time 300</dd>
-
<dd>Denaturing: Temp 95, Time 30</dd>
+
<dd>Denaturing: Temp 95&deg;C, Time 30</dd>
-
<dd>Anneal: Temp 54, Time 30</dd>
+
<dd>Anneal: Temp 54&deg;C, Time 30</dd>
-
<dd>Extend: Temp 72, Time 120</dd>
+
<dd>Extend: Temp 72&deg;C, Time 120</dd>
-
<dd>Final Step: Temp 72, Time 420</dd>
+
<dd>Final Step: Temp 72&deg;C, Time 420</dd>
-
<dd>Final Hold: Temp 4</dd>
+
<dd>Final Hold: Temp 4&deg;C</dd>
<dd>Cycles: 30</dd></dl></li>
<dd>Cycles: 30</dd></dl></li>
<li>Prepared overnight cultures of MAK31:TRP1 and VPS75:TRP1 (3, 6)</li></ul>
<li>Prepared overnight cultures of MAK31:TRP1 and VPS75:TRP1 (3, 6)</li></ul>
Line 428: Line 440:
<li>Miniprepped TRP and LEU</li>
<li>Miniprepped TRP and LEU</li>
<li><dl><dt>Nanodrop results:</dt>
<li><dl><dt>Nanodrop results:</dt>
-
<dd>TRP: 9.9 ng/uL</dd>
+
<dd>TRP: 9.9 ng/&mu;L</dd>
-
<dd>LEU: 122.2 ng/uL</dd></dl></li>
+
<dd>LEU: 122.2 ng/&mu;L</dd></dl></li>
<li>prepared definitions and big ideas for meeting</li></ul><br>  
<li>prepared definitions and big ideas for meeting</li></ul><br>  
Line 454: Line 466:
<li>Put diluted yeast culture in shaker at 11:35am.</li>
<li>Put diluted yeast culture in shaker at 11:35am.</li>
<li>Purified and nanodropped PCR product  
<li>Purified and nanodropped PCR product  
-
<dl><dd>EL1: 9.2 ng/uL</dd>
+
<dl><dd>EL1: 9.2 ng/&mu;L</dd>
-
<dd>EL2: 4.8 ng/uL</dd>
+
<dd>EL2: 4.8 ng/&mu;L</dd>
-
<dd>EL3: 2.7 ng/uL</dd>
+
<dd>EL3: 2.7 ng/&mu;L</dd>
-
<dd>EL4: 13.6 ng/uL</dd></dl></li>
+
<dd>EL4: 13.6 ng/&mu;L</dd></dl></li>
<li>Transformed yeast strains VT3 + EL1, VT6 + EL2, MT7 + EL3, MTB + EL4</li></ul><br>
<li>Transformed yeast strains VT3 + EL1, VT6 + EL2, MT7 + EL3, MTB + EL4</li></ul><br>
<img src=" https://static.igem.org/mediawiki/2014/c/c6/CU_729_no_UV.jpg " width="200" />
<img src=" https://static.igem.org/mediawiki/2014/c/c6/CU_729_no_UV.jpg " width="200" />
Line 470: Line 482:
<li>Prepared for tomorrow's presentation</li>
<li>Prepared for tomorrow's presentation</li>
<li>Researched assaying protocol (x) (x) (x)</li>
<li>Researched assaying protocol (x) (x) (x)</li>
-
<li>Restreaked W303A and W303alpha for assaying on Friday (1:00 pm)</li></ul>
+
<li>Restreaked W303A and W303&alpha; for assaying on Friday (1:00 pm)</li></ul>
<br>
<br>
For tomorrow: finish presentation, make more YPD plates, prepare for assay <br>
For tomorrow: finish presentation, make more YPD plates, prepare for assay <br>
Line 483: Line 495:
<table>  
<table>  
<tr><td>Master Mix</td><td class="right">1x</td><td class="right">9x</td></tr>
<tr><td>Master Mix</td><td class="right">1x</td><td class="right">9x</td></tr>
-
<tr><td>10x ThermoPol Buffer</td><td  class="right">2.5 uL</td><td class="right">22.5 uL</td></tr>
+
<tr><td>10x ThermoPol Buffer</td><td  class="right">2.5&mu;L</td><td class="right">22.5&mu;L</td></tr>
-
<tr><td>Primers (Forward & Reverse)</td><td class="right">5 uL</td><td  class="right">45 uL</td></tr>
+
<tr><td>Primers (Forward & Reverse)</td><td class="right">5&mu;L</td><td  class="right">45&mu;L</td></tr>
-
<tr><td>10mM dNTP</td><td  class="right">0.25 uL</td><td  class="right">2.25 uL</td></tr>
+
<tr><td>10mM dNTP</td><td  class="right">0.25&mu;L</td><td  class="right">2.25&mu;L</td></tr>
-
<tr><td>Template</td><td  class="right">5 uL</td><td></td></tr>  
+
<tr><td>Template</td><td  class="right">5&mu;L</td><td></td></tr>  
-
<tr><td>Taq DNA Polymerase</td><td  class="right">0.5 uL</td><td  class="right">4.5 uL</td></tr>
+
<tr><td>Taq DNA Polymerase</td><td  class="right">0.5&mu;L</td><td  class="right">4.5&mu;L</td></tr>
-
<tr><td>ddH2O</td><td class="right">11.75 uL</td><td class="right">105.75</td></tr>
+
<tr><td>ddH2O</td><td class="right">11.75&mu;L</td><td class="right">105.75&mu;L</td></tr>
-
<tr><td>Total</td><td  class="right">25 uL</td><td class="right">180</td></tr></table></li>
+
<tr><td>Total</td><td  class="right">25&mu;L</td><td class="right">180&mu;L</td></tr></table></li>
<li>Poured YPD plates (two 250mL bottles)</li>
<li>Poured YPD plates (two 250mL bottles)</li>
<li>Made four 1% agarose gels</li>
<li>Made four 1% agarose gels</li>
-
<Li>Ran gels of PCR samples.
+
<Li>Ran gels of PCR samples.<br><br>
 +
<img src=" https://static.igem.org/mediawiki/2014/c/c1/CU_731_Gel_Run_MT71_and_VT62.jpg " width="350" />
 +
<img src=" https://static.igem.org/mediawiki/2014/0/04/CU_731_Gel_Run_MTB1_and_MTB2.jpg " width="350" /><br>
<dl><dd>Gel 1 Wells: 1. blank ; 2. 250bp ladder ; 3. MTB1(1) ; 4. MTB1(2) ; 5. MTB2(1) ; 6. MTB2(2). </dd>
<dl><dd>Gel 1 Wells: 1. blank ; 2. 250bp ladder ; 3. MTB1(1) ; 4. MTB1(2) ; 5. MTB2(1) ; 6. MTB2(2). </dd>
<dd> Gel 2 Wells: 1. Blank ; 2. 250bp ladder ; 3. MT71(1) ; 4. MT71(2) ; 5. VT62(1) ; 6. VT62(2)</dd>
<dd> Gel 2 Wells: 1. Blank ; 2. 250bp ladder ; 3. MT71(1) ; 4. MT71(2) ; 5. VT62(1) ; 6. VT62(2)</dd>
Line 500: Line 514:
<dd> There were bright bands outside the ladder.</dd></dl></li>
<dd> There were bright bands outside the ladder.</dd></dl></li>
<li>Put 6mL inoculations of 1294, 1296, 1297, W303A, W303alpha into roller</li></ul>
<li>Put 6mL inoculations of 1294, 1296, 1297, W303A, W303alpha into roller</li></ul>
-
<br>
+
 
-
<img src=" https://static.igem.org/mediawiki/2014/c/c1/CU_731_Gel_Run_MT71_and_VT62.jpg " width="200" />
+
-
<img src=" https://static.igem.org/mediawiki/2014/0/04/CU_731_Gel_Run_MTB1_and_MTB2.jpg " width="200" /><br>
+
For tomorrow: count yeast cells<br>
For tomorrow: count yeast cells<br>
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Latest revision as of 00:48, 18 October 2014

Cooper Union 2014 iGEM

Programmable Lifespan Timer


7/1/14

(Nolana)
  • Yeast transformed inoculated overnight cultures of 1880, 1882, and W303a
  • PCR'd 4 samples for yeast deletion cassettes: MAK31+TRP1 (MT), MAK31+LEU2 (ML), VPS75+TRP1 (VL), VPS75+LEU2 (VL)
  • Took photos of yeast plates to check for growth (1294, 1296, 1297, 1300, and W303alpha); restreaked all plates

(Jae Ho)

Yeast Transformation>>Follows Protocol
PCR plasmid purification skipped due to time restraints.
AMT, AVT, 82VL, 80ML Transformations prepared, and plated. w303A, 1882, 1880 Negative control plates also prepared.


For tomorrow: run gel of PCR samples

7/2/14

(Nolana, Jae Ho)
  • restreaked yeast plates from last week (the ones that were likely to be TRP);
    6 Plates restreaked at day 4 after day 1 (faint): W303α+TRP1-1, W303α negative control, W303α+TRP1-3
  • Photos of yeast plates/restreaked: 1300, 1294, 1296,1297, w303α
    Due to deletion of EST2, 1294,1296,1297 are fading:dying
  • New transformation done by prof. Medvedik: wrong plates on original transformation
  • Ran gel with yesterday's PCR samples (MT, ML, VT, VL) with one of the De Novo group's pet28+TdT samples. Used VersaLadder.


    Wells: 1. blank ; 2. ladder ; 3. VT ; 4. VL ; 5. MT ; 6. ML ; 7. pET28+TdT

    Sizes expected: 1074 for VT and MT, 2415 VL and ML
  • Results: we had to stain the gel with ethidium bromide because everything was too faint at first.
    VL and ML had approximately 2kb; VT and MT had approximately 1kb --> good results!
    However, there were other bands that showed along with the PCR amplification -- maybe raise temperature to 56°C instead of 54°C.


For tomorrow: run PCR with same samples, but with different temperature

7/3/14

(Jae Ho)
PCR machine not available, unable to do PCR
Restreaked cultures and took photos
Restreaked successful transformation colonies: Mak31+TRP1/VPS75+TRP1

For later: PCR EST1+LEU2, EST1+TRP1
Out of TRP plates



7/7/14


PCR: EST1+TRP1, EST1+LEU2
Culture preps: W303A, W303α, 1300, 1296
New YPD plates made
Plates struck
Gel Run with 1% gel and 1k ladder:


Two showed nothing while the third ET showed multiple bands.

Could be contamination in sample/annealing temperature problem (54°C->56&degC, maybe try 58°C)




Tomorrow: Transformation

7/8/14

(Nolana)
  • Ran 1% gel of PCR samples ET1, ET2, EL1, ET2.

    Wells: 2. BioLabs 1kb ladder ; 3. EL1 ; 3. EL2 ; ET1 ; ET2
  • Gel results were faint, so we stained the gel in ethidium bromide for 15 minutes.
    Expected sizes -- ET: 1074 ; EL: 2415.
    Results: the ET sizes matched but the EL did not -- maybe the plasmid template is contaminated;
    miniprep LEU2 plasmid again?
  • Checked and restreaked yeast plates to check for growth
  • Yeast transformation of W303α, W303a, 1300, 1296
  • 1296 discarded for transformation
  • Knockout of EST1+TRP1/LEU2 for other strains in progress



For tomorrow: Miniprep TRP, LEU
Check MAK31 and VPS75 knock plates by colony PCR
Make TRP and LEU plates

7/9/14

(Lily)
  • Checked and restruck yeast plates
  • Left culture overnight for miniprep tomorrow (will do!)

(Nolana)
  • Made TRP- and LEU- selective yeast plates
  • helped Dionne run her PCR samples on a 1.5% gel (wells: 1. VersaLadder ; 2-7:(1)-(6) ; 8. (8) )
  • ran PCR overnight (colony PCR for 2 samples each of MAK31::TRP1, MAK31::LEU2, VPS75::TRP1, VPS75::LEU2 and 2 samples each of ET, EL)



For tomorrow: re-miniprep plasmids for pFA6a-TRP1, pFA6a-LEU3MX6;
Run gel for colony PCR samples
Purify PCR samples of knockout cassettes
Check and restreak yeast plates

7/10/14

(Nolana)
  • Miniprepped pFA6a-TRP1 and pFA6a-LEU2MX6 plasmid templates
  • Nanodropped miniprep samples:
    TRP1: 298.4 ng/μL
    LEU2: 163.8 ng/μL
  • Yeast plates were restruck and photos were taken for growth monitoring
  • PCR'ed two samples each of EST1+LEU2, EST1+TRP1 for PCR purification and then yeast transformation tomorrow.
    PCR conditions: program 333, temperature 54°C, 180 seconds extension time, 30 cycles
  • Ran two 1% gels of yesterday's PCR product:
    gel 1 wells: 1-3: blank ; 4. MT1 ; 5: ML1 ; 6. VT1 ; 7. VL1 ; 8. Biolabs 100bp ladder
    gel 2 wells: 1-3: blank ; 4. MT2 ; 5: ML2 ; 6. VT2 ; 7. VL2 ; 8. Biolabs 100bp ladder
  • Inoculated yeast strains in YPD for overnight culture for transformation


For tomorrow: purify PCR products and the yeast transform strains 1300, W303A, W303alpha

7/11/14

(Jae Ho)
Transformation Not done due to lack of culture: Reculture on Sunday
PCR purification results: near 0 concentration: Redo PCR on Sunday
Gels ran again

gel 1 wells: 1blank ; 2. ladder 3. MT1 ; 4: ML1 ; 5. VT1 ; 6. VL1
gel 2 wells: 1blank ; 2. Ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2
Plates restruck, photos taken


For Monday: Tranformation, PCR purification

7/14/14


PCR machine failure
Yeast plates restruck, photos taken
Overnight cultures of 1300. W303a. W303A remade
Gel run


gel 1 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML1 ; 5. VT1 ; 6. VL1; 7 versa ladder
gel 2 wells: 1blank ; 2. 100 base ladder 3. MT2 ; 4: ML2 ; 5. VT2 ; 6. VL2 ; 7.versa ladder
Gel 2: the samples ran off so results were unobtainable.

Redoing PCR of EL and ET on the other machine.


Tomorrow: Check PCR (Gel/ purification), Transformation of 1300, W303a, W303A if PCR is successful.

7/15/14

  • Checked gel pictures from last gel run
    Expected sizes of gene w/out knockout:
    MAK31: 381 bp
    VPS75: 406 bp
    Expected sizes with knockout:
    MAK31: 285 bp
    VPS75: 275 bp
  • Ran PCR of MT, ML, VT, VL (one regular, one universal sample) on the new OpenPCR machine, program 334:
    Initial Step: Temp 95°C, Time 300
    Anneal: Temp 56°C, Time 30
    Extend: Temp 72°C, Time 30
    Final Step: Temp 72°C, Time 420
    Final Hold: Temp 4°C
    Cycles: 30
  • Ran two 1% gels (10uL PCR product, 2 uL 10x loading dye)


    Gel 1 wells: 1. blank ; 2. 100bp ladder ; 3. MT1 ; 4. ML1 ; 5. VT1 ; 6. VL1
    Gel 2 wells: 1. blank ; 2. 100bp ladder ; 3. MT2 ; 4. ML2 ; 5. VT2 ; 6. VL2
  • Gel results: MAK31 and VPS75 did not get deleted from the yeast colonies (no bright bands on gel 2)
  • Ran PCR again with same settings, but with new colonies


For tomorrow: run gel

07/16/14

  • Made four 1% gels and ran them with the following:
    Colony 3: A-D
    Colony 4: E-G
  • Ran gels of all PCR samples for genes without knockouts (samples A-H)


    Gel run
    gel 1.1 wells: 1blank ; 2. 250 base ladder ; 3. (A1) MT1 ; 4: (B1) ML1 ; 5. (C1) VT1 ; 6. (D1) VL1
    gel 1.2 wells: 1blank ; 2. 250 base ladder ; 3. (E1) MT2 ; 4: (F1) ML2 ; 5. (G1) VT2 ; 6. (H1) VL2
  • Ran gels of all PCR samples for genes with universal primers (samples A-H)



    Gel run
    gel 2.1 wells: 1blank ; 2. 250 base ladder 3. (A2) MT1 ; 4: (B2) ML1 ; 5. (C2) VT1 ; 6. (D2) VL1
    gel 2.2 wells: 1blank ; 2. 250 base ladder 3. (E2) MT2 ; 4: (F2) ML2 ; 5. (G2) VT2 ; 6. (H2) VL2
  • Results:
    gels 1.1 and 1.2 all had bands -- this indicates that the genes were not deleted
    gel 2.2 had no bands -- this goes along with the results from gel 1.1 and 1.2
    gel 2.1 had one very bright VT band -- streak out this colony to double check later?

For tomorrow: screen more colonies! If gels still show no deletions, then maybe do yeast transformation on Friday.

7/17/14

  • Colony PCR
    Colony 5: A-D
    Colony 6: E-H
  • Ran gels of all PCR samples for genes without knockouts (A-H 3)


    Gel run
    gel 1 wells: 1blank ; 2. 250 base ladder ; 3. (A3) MT1 ; 4: (B3) ML1 ; 5. (C3) VT1 ; 6. (D3) VL1
    gel 2 wells: 1blank ; 2. 250 base ladder ; 3. (E3) MT2 ; 4: (F3) ML2 ; 5. (G3) VT2 ; 6. (H3) VL2
  • Ran gels of all PCR samples for genes with universal primers (samples A-H 4)

    Gel run
    gel 3 wells: 1blank ; 2. 250 base ladder 3. (A4) MT1 ; 4: (B4) ML1 ; 5. (C4) VT1 ; 6. (D4) VL1
    gel 4 wells: 1blank ; 2. 250 base ladder 3. (E4) MT2 ; 4: (F4) ML2 ; 5. (G4) VT2 ; 6. (H4) VL2
  • Results:
    bands for VPS75:: TRP1 for colonies 5 and 6 showed. possible knockout
  • Restreaked VPS75:: TRP1 of colonies 3, 5, and 6

For tomorrow: screen more colonies! MAK31 colonies
Check restreaked colonies

7/18/14:

  • Colony PCR'ed MAK31::TRP1 deletion strain. 10 samples: 5 samples from Plate A (A7-A11), 5 samples from Plate B (B1-B5).
    PCR settings: program 334, anneal temp: 56, extension time: 30 sec.
  • Made two 1% agarose gels


    Ran gels
    gel 1 wells: 1. blank ; 2. Versa ladder ; 3-6. A7-10 ; 7-8. Shoshana and Devora's samples
    gel 2 wells: 1 blank ; 2. Versa ladder ; 3-7. B1-5 ; 8. A11
  • Results: gel 1 had one faint band at A7, we stained the gel in 400 mL H2O and 500μL ethidium bromide for 15 minutes.
    After staining, the band was still faint. All the Plate B samples on gel 2 had successful knockouts, but we realized the samples were taken from one streaked out colony.
  • Streaked out 2 YPD plates for the MAK31:TRP1 deletion: 1 plate B colony, A7
  • Overnight PCR of Plate B colony to double-check deletion: one sample with universal primer, one sample with gene check primer

For Monday: check the MAK31 colonies and the VPS colonies that were struck yesterday.
Prepare for new transformations for those strains with EST1.

7/21/14

  • Made four 1% agarose gels
  • ran PCR of VT colonies with possible knockouts that were streaked out last week. 6 samples: 2 of each colony (one with universal primer, one with gene check primer): colonies 3, 5, 6 using the OpenPCR program 334.
  • Ran gel of last week's MT samples: 2 samples: one with universal primer, one with gene check primer.


    Wells: 1. blank ; 2. Versa ladder ; 3. universal ; 4. gene check
  • Results: there were bands for both lanes on the gel, which corresponded to their respective sequence sizes (universal: 275, gene check: 406) -- maybe yeast strain is diploid?
  • Ran gel of VT colonies.


    Wells: 1. Versa ladder ; 2. 3R ; 3. 5R ; 4. 6R ; 5. 3U ; 6. 5U ; 7. 6U
  • Results: bands were faint, stained gel in 200mL H2O+250μL ethidium bromide. After staining, confirmed that 2 colonies had knockouts (3 and 6)
  • Streaked out three plates of previous W303α transformation
  • Streaked out original 1808 colony (pre-transformation)


For tomorrow: make more YPD plates, check MAK31 plates again, prepare for yeast transformation

7/22/14:

  • Made YPD plates
  • restreaked 1880, VPS75:TRP1 colonies 3, 6 for testing UV phenotype
  • Ran overnight PCR samples of EST1+LEU2 for tomorrow (purification and yeast transformation
    Program: PCR for ~1-2kb 54c
    Initial Step: Temp 95°C, Time 300
    Denaturing: Temp 95°C, Time 30
    Anneal: Temp 54°C, Time 30
    Extend: Temp 72°C, Time 120
    Final Step: Temp 72°C, Time 420
    Final Hold: Temp 4°C
    Cycles: 30
  • Prepared overnight cultures of MAK31:TRP1 and VPS75:TRP1 (3, 6)

For tomorrow: yeast transformation, PCR purification, miniprep LEU2

For some later date: make biobrick parts for VPS75 deletion

07/23/14

  • Yeast transformation with EST1 of MAK31:TRP1 and VPS75:TRP1 (3, 6)
  • Put dilution in shaker at 11:07 am
  • PCR purified yesterday's samples (3 samples of EST1::LEU2)
  • Checked MAK31 and VPS75 BioBrick primers for Prof. Medvedik to order
  • Counted cells of MAK31 and VPS75
  • Step 14 of transformation
    MT : EL1
    VT3 : EL2
    VT6 : EL3
  • Streaked out 1880, VPS75:TRP1 (3, 6) on plate.
    Exposed to UV light on low setting for two seconds to confirm VPS75 phenotype (sensitivity to UV light)
  • Inoculate a culture of LEU2 plasmid for miniprep tomorrow

7/24/14

  • Miniprepped TRP and LEU
  • Nanodrop results:
    TRP: 9.9 ng/μL
    LEU: 122.2 ng/μL
  • prepared definitions and big ideas for meeting

7/28/14:

  • Checked transformation plates: nothing grew except for the VPS75 Colony 3 plates, which had grown fungus because of a contamination in the YPD media
  • Colony PCR'ed 3 samples of the first EST1 transformation with the universal primer to check for knockouts (OpenPCR program 334)
  • Replicated 4 plates of 1880 strain+VPS75 knockouts. UV- shocked 3 plates on high: 10 sec, 30 sec, 1 min.
  • Ran 1% gel of samples.
    Wells: 1. blank ; 2. Versa ladder 3. plate 6 ; 4. plate 7 ; 5 plate 8.
    Results: there were no bands on the gel, meaning that there were no knockouts.
    Expected sizes of EST1 knockout:
    with universal primer: 205 bp
    with gene check primer: 500 bp
  • Inoculated cultures for tomorrow's transformation
For tomorrow: PCR EST1 deletion cassettes, purify PCR product, yeast transformation, check UV plates

7/29/14

  • PCR'ed EST1+LEU2 for purification and transformation
  • Put diluted yeast culture in shaker at 11:35am.
  • Purified and nanodropped PCR product
    EL1: 9.2 ng/μL
    EL2: 4.8 ng/μL
    EL3: 2.7 ng/μL
    EL4: 13.6 ng/μL
  • Transformed yeast strains VT3 + EL1, VT6 + EL2, MT7 + EL3, MTB + EL4


For tomorrow: make more LEU- plates

7/30/14

  • Made more LEU- plates (1 bottle of 400 mL)
  • Prepared for tomorrow's presentation
  • Researched assaying protocol (x) (x) (x)
  • Restreaked W303A and W303α for assaying on Friday (1:00 pm)

For tomorrow: finish presentation, make more YPD plates, prepare for assay

7/31/14

  • Checked EST1 transformations: no growth on VT6 plate 1, MT7 plate 2, VT3 plate 1. There were non-yeast growths on MT7 plate 1 and VT3 plate 2
  • Restreaked all 5 yeast colonies of VT3 plate 2
  • Chose 2 colonies each for colony PCR: MTB plate 1, MTB plate 2, MT7 plate 1, VT6 plate 2
  • Instead of using PCR tubes with beads, we used a standard PCR reaction:
    Master Mix1x9x
    10x ThermoPol Buffer2.5μL22.5μL
    Primers (Forward & Reverse)5μL45μL
    10mM dNTP0.25μL2.25μL
    Template5μL
    Taq DNA Polymerase0.5μL4.5μL
    ddH2O11.75μL105.75μL
    Total25μL180μL
  • Poured YPD plates (two 250mL bottles)
  • Made four 1% agarose gels
  • Ran gels of PCR samples.


    Gel 1 Wells: 1. blank ; 2. 250bp ladder ; 3. MTB1(1) ; 4. MTB1(2) ; 5. MTB2(1) ; 6. MTB2(2).
    Gel 2 Wells: 1. Blank ; 2. 250bp ladder ; 3. MT71(1) ; 4. MT71(2) ; 5. VT62(1) ; 6. VT62(2)
    Gel Results
    we used too much ladder (wrong concentration).
    There were very faint bands -- maybe redo PCR with raised temperature.
    There were bright bands outside the ladder.
  • Put 6mL inoculations of 1294, 1296, 1297, W303A, W303alpha into roller
For tomorrow: count yeast cells