Team:Grenoble/Biology/Notebook/June/week 28

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<a href="https://2012.igem.org/Team:Grenoble/Biology/Notebook/July">week 27</a>
 
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<a href="https://2012.igem.org/Team:Grenoble/Biology/Notebook/June/week_28">week 28</a>
 
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<a href="https://2012.igem.org/Team:Grenoble/Biology/Notebook/June/week_29">week 29</a>
 
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<a href="https://2012.igem.org/Team:Grenoble/Biology/Notebook/June/week_30">week 30</a>
 
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<br/>
 
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<br/>
 
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<h1> Week 28: July 09<span class="exposant">th</span> to July 15<span class="exposant">th</span> </h1>
 
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<h2> Goal of the week </h2>
 
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we wanted to recover and amplify the biobricks involved in our genetic networks:
 
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<ul>
 
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<li>pAra/Bad_RBS_GFP (1300bp)</li>
 
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<li>RBS_Cya (2600bp)</li>
 
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<li>pLAC (100bp)</li>
 
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<li>fha (80bp)</li>
 
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<li>eCFP (800bp)</li>
 
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<li>pLAC_RBS (120bp)</li>
 
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<li>RsmA (200bp)</li>
 
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<li>rsmY (170bp)</li>
 
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<li>pSB1A3 (2400bp)</li>
 
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<li>pSB4K5 (2400bp)</li>
 
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<li>pSB3C5 (2400bp)</li>
 
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</ul>
 
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We also planned to realise the gibson assemblies for the first constructions.
 
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<br/><br/>
 
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<h2> Monday, July 09<span class="exposant">th</span>:</h2>
 
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Precultured cells are prepared:
 
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<ul>
 
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<li>Strains = BW25113 WT and BW25113 cya- pAra/Bad </li>
 
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<li>Conditions = LB liquid medium, 37°C, 200rpm, overnight </li>
 
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</ul>
 
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<br/>
 
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<h2>Tuesday, July 10<span class="exposant">th</span>:</h2>
 
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For the PCRs, we changed the enzyme from GoTaq to High Fidelity (HF) Phusion.<br/>
 
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We did some colony PCR with a HF Phusion enzyme (protocol) to amplify:
 
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<ul>
 
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<li>fha1, RsmA, rsmY and pSB1A3 from iGEM Grenoble 2011 glycerol stock.</li>
 
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<li>pAra/Bad_RBS_GFP from BW25113 cya- pAra/Bad precultured cells.</li>
 
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<li>RBS_Cya from BW25113 WT precultured cells.</li>
 
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</ul>
 
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We did the PCR both with and without DMSO (Amplification of difficult targets, such as those with GC-rich sequences or secondary structure, may be improved by the presence of additives such as DMSO).<br/>
 
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<br/>
 
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To separate the PCR products, we prepared two gels:
 
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<ul>
 
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<li>a 1.3% TAE agarose gel, for the small fragments: RsmA, fha1 and rsmY (length < 1000bp)</li>
 
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<li>a 0.8% TAE agarose gel, for the big fragments: pSB1A3, RBS_Cya, and pAra/Bad_RBS_GFP (length > 1000bp)</li>
 
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</ul>
 
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<br/>Migration conditions = 50V during 1h15.<br/>
 
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We used EtBr to reveal the DNA fragments.<br/>
 
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<center><img src="https://static.igem.org/mediawiki/2012/b/b6/120710.jpg" alt="photo_gel_4"/></center>
 
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<u>Migration result for the 1.3% TAE agarose gel (small fragments)</u><br/>
 
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      <i>(the DNA ladder scale is in kb)</i><br/>
 
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Lane 1: DNA ladder 100bp (biolabs)<br/>
 
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Lane 2 and 3: fha1 PCR product<br/>
 
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Lane 4 and 5: RsmA PCR product<br/>
 
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Lane 6 and 7: rsmY PCR product<br/>
 
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Lane 8 and 9: fha1 PCR product (DMSO)<br/>
 
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Lane 10 and 11: RsmA PCR product (DMSO)<br/>
 
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Lane 12: rsmY PCR product (DMSO)<br/>
 
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Lane 13: DNA ladder 100bp (biolabs)<br/>
 
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<br/>
 
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<center><img src="https://static.igem.org/mediawiki/2012/4/4e/120710_%282%29.jpg" alt="photo_gel_5"/></center>
 
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<u>Migration result for the 0.8% TAE agarose gel (big fragments)</u><br/>
 
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            <i> (the DNA ladder scale is in kb)</i><br/>
 
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Lane 1: DNA ladder 1kb (biolabs)<br/>
 
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Lane 2 and 3: RBS_Cya PCR product<br/>
 
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Lane 4 and 5: pSB1A3 PCR product<br/>
 
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Lane 6 and 7: pAra/Bad_RBS_GFP PCR product<br/>
 
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Lane 8 and 9: RBS_Cya PCR product (DMSO)<br/>
 
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Lane 10 and 11: pSBA13 PCR product (DMSO)<br/>
 
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Lane 12: pAra/Bad_GFP PCR product (DMSO)<br/>
 
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Lane 13: DNA ladder 1kb (biolabs)<br/>
 
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<br/>
 
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There was a migration problem on the second gel (DNA ladder migration was not right) and we only saw primer dimer bands. There was a PCR condition problem.<br/>
 
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<br/>
 
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Precultured cells were prepared:
 
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<ul>
 
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<li>Strains = BW25113 WT.</li>
 
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<li>Conditions = LB liquid medium, 37°C, 200rpm, overnight.</li>
 
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</ul>
 
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<h2> Wednesday, July 11<span class="exposant">th</span>:</h2>
 
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</section>
 
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Latest revision as of 14:56, 6 August 2012