Difference between revisions of "Team:Yale/notebook"

 
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         <li><a href="https://2015.igem.org/Team:Yale/notebook" alt="Notebook">Notebook</a></li>
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         <li class="submenu"><a href="notebook">Notebook</a>
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          <ul>
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            <li><a href="https://2015.igem.org/Team:Yale/notebook" alt="Weekly">Weekly</a></li>
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            <li><a href="https://static.igem.org/mediawiki/2015/f/fb/Yale_iGEM_Project_Summary_2015.pdf" alt="PDF Summary">PDF Summary</a></li>
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         <li class="submenu"><a href="collaborations">Collaborations</a></li>
 
         <li class="submenu"><a href="collaborations">Collaborations</a></li>
 
         <li class="submenu"><a href="practices">Human Practices</a>
 
         <li class="submenu"><a href="practices">Human Practices</a>
 
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            <li><a href="https://2015.igem.org/Team:Yale/practices#video" alt="Documentary">Documentary</a></li>
 
 
             <li><a href="https://2015.igem.org/Team:Yale/practices#ssri" alt="SSRI">SSRI</a></li>
 
             <li><a href="https://2015.igem.org/Team:Yale/practices#ssri" alt="SSRI">SSRI</a></li>
 
             <li><a href="https://2015.igem.org/Team:Yale/practices#lgbtq" alt="LGBTQ Survey">LGBTQ Survey</a></li>
 
             <li><a href="https://2015.igem.org/Team:Yale/practices#lgbtq" alt="LGBTQ Survey">LGBTQ Survey</a></li>
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         <li class="submenu"><a href="team">Team</a>
 
         <li class="submenu"><a href="team">Team</a>
 
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             <li><a href="https://2015.igem.org/Team:Yale/team" alt="People">People</a></li>
             <li><a href="https://2015.igem.org/Team:Yale/team#acknowledgements" alt="Acknowledgements">Acknowledgements</a></li>
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             <li><a href="https://2015.igem.org/Team:Yale/Attributions" alt="Acknowledgements">Attributions</a></li>
 
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        <li class="submenu"><a href="standards">Standards</a>
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        <li class="submenu"><a href="https://2015.igem.org/Team:Yale/standards">Standard Pages</a>
 
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             <li><a href="https://2015.igem.org/Team:Yale/standards#gold" alt="Gold">Gold</a></li>
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            <li><a href="https://2015.igem.org/Team:Yale/standards" alt="Gold">Standard Pages</a></li>
             <li><a href="https://2015.igem.org/Team:Yale/standards#silver" alt="Silver">Silver</a></li>
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             <li><a href="https://2015.igem.org/Team:Yale/standards#gold" alt="Gold">Gold Standards</a></li>
             <li><a href="https://2015.igem.org/Team:Yale/standards#bronze" alt="Bronze">Bronze</a></li>
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       <p>Our rhizobium transformation experiments gave us mixed results. Using electroporation, R. tropici was able to take up the KT230 plasmid, but S. meliloti 356, 370, and 371 demonstrated kan and spec resistance and we were not able to determine whether the transformation was successful for those strains. We also experimented with conjugation as an alternative transformation method. We found a protocol for conjugating E. coli to UTEX 2973 and began to incubate E. coli containing pKT230.2 When UTEX 2973 reaches OD750 0.5, we will proceed with conjugation.</p>
 
       <p>Our rhizobium transformation experiments gave us mixed results. Using electroporation, R. tropici was able to take up the KT230 plasmid, but S. meliloti 356, 370, and 371 demonstrated kan and spec resistance and we were not able to determine whether the transformation was successful for those strains. We also experimented with conjugation as an alternative transformation method. We found a protocol for conjugating E. coli to UTEX 2973 and began to incubate E. coli containing pKT230.2 When UTEX 2973 reaches OD750 0.5, we will proceed with conjugation.</p>
 
       <p>We performed several rhizobium antibiotic resistance assays to determine whether our strains of rhizobium have natural resistance to certain antibiotics. The results suggested that none of our strains have kanamycin resistance, but R. tropici and S. meliloti 371 have spectinomycin resistance. We also performed a rifampicin assay to determine whether we could eventually use MAGE to induce resistance to rifampicin in rhizobium. The assay worked with 2x1010 cells, but even 20 uL/mL rifampicin was below the limit of detection (see Fig. 1). Our goal moving forward is to redo this assay at lower concentrations.</p>
 
       <p>We performed several rhizobium antibiotic resistance assays to determine whether our strains of rhizobium have natural resistance to certain antibiotics. The results suggested that none of our strains have kanamycin resistance, but R. tropici and S. meliloti 371 have spectinomycin resistance. We also performed a rifampicin assay to determine whether we could eventually use MAGE to induce resistance to rifampicin in rhizobium. The assay worked with 2x1010 cells, but even 20 uL/mL rifampicin was below the limit of detection (see Fig. 1). Our goal moving forward is to redo this assay at lower concentrations.</p>
       <p class="text-center"><img src="http://client.cameronyick.us/igem/assets/img/journal/pigeon.jpg"></p>
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       <p class="text-center"><img src="https://static.igem.org/mediawiki/2015/thumb/7/7b/Antibiotic_assay_rhizo.jpeg/1600px-Antibiotic_assay_rhizo.jpeg"></p>
 
       <p>We also met with Professor Dellaporta, one of our PIs, about the possibility of using ligation-independent cloning (LIC) as an alternative to Gibson Assembly. With LIC, the BsaI T4 DNA polymerase generates long complimentary sticky ends between the vector and insert and eliminates the need for ligase. The advantage is that one LIC cloning vector can be used repeatedly to build many promoter and beta homolog constructs without PCR amplifying the large vector backbone each time. However, we would need to order new primers and spend a week constructing the LIC vector.</p>
 
       <p>We also met with Professor Dellaporta, one of our PIs, about the possibility of using ligation-independent cloning (LIC) as an alternative to Gibson Assembly. With LIC, the BsaI T4 DNA polymerase generates long complimentary sticky ends between the vector and insert and eliminates the need for ligase. The advantage is that one LIC cloning vector can be used repeatedly to build many promoter and beta homolog constructs without PCR amplifying the large vector backbone each time. However, we would need to order new primers and spend a week constructing the LIC vector.</p>
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf#page=16" class="file__link">Go to the Lab Notebook</a></p>
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf#page=16" class="file__link">Go to the Lab Notebook</a></p>
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       <p>We were able to PCR amplify three rhizobium-specific inducible promoters: melA, bacA, and nodF. We also have the Anderson constitutive promoters from the iGEM registry, which we will use for both cyanobacteria and Rhizobia. For both organisms, we started amplifying our control genes of interest (GFP for Rhizobia, citrine for cyanobacteria) with overhangs to the promoters.</p>
 
       <p>We were able to PCR amplify three rhizobium-specific inducible promoters: melA, bacA, and nodF. We also have the Anderson constitutive promoters from the iGEM registry, which we will use for both cyanobacteria and Rhizobia. For both organisms, we started amplifying our control genes of interest (GFP for Rhizobia, citrine for cyanobacteria) with overhangs to the promoters.</p>
 
       <p>Much of our transformations this week were in preparation for Exonuclease and Ligation Independent Cloning (ELIC) or for amplification of broad host range plasmids into E. coli. We are considering using ELIC as a backup or more efficient alternative to Gibson assembly. For ELIC, we chose to work with the plasmid pZE21G as a control experiment; this plasmid along with the chromoprotein amilCP should be able to be successfully assembled. Additionally, we have been experimenting with natural transformation in cyanobacteria and are still waiting for the transformation cultures to grow up more before forming conclusions. Regarding electroporation in E. coli, we are still troubleshooting transformations with our two main plasmids pKT230 and k125000.</p>
 
       <p>Much of our transformations this week were in preparation for Exonuclease and Ligation Independent Cloning (ELIC) or for amplification of broad host range plasmids into E. coli. We are considering using ELIC as a backup or more efficient alternative to Gibson assembly. For ELIC, we chose to work with the plasmid pZE21G as a control experiment; this plasmid along with the chromoprotein amilCP should be able to be successfully assembled. Additionally, we have been experimenting with natural transformation in cyanobacteria and are still waiting for the transformation cultures to grow up more before forming conclusions. Regarding electroporation in E. coli, we are still troubleshooting transformations with our two main plasmids pKT230 and k125000.</p>
      <p class="text-center"><img src="http://client.cameronyick.us/igem/assets/img/journal/pigeon.jpg"></p>
 
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf#page=25" class="file__link">Go to the Lab Notebook</a></p>
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf#page=25" class="file__link">Go to the Lab Notebook</a></p>
 
       <h4 class="week_log">Entry for week<a href="#" data-reveal-id="week1">-1</a><a href="#" data-reveal-id="week2">1</a><a href="#" data-reveal-id="week3">2</a><a href="#" data-reveal-id="week4">3</a><a href="#" data-reveal-id="week5">4</a><a href="#" data-reveal-id="week6">5</a><a href="#" data-reveal-id="week7">6</a><a href="#" data-reveal-id="week8">7</a><a href="#" data-reveal-id="week9">8</a><a href="#" data-reveal-id="week10">9</a><a href="#" data-reveal-id="week11">10</a><a href="#" data-reveal-id="week12">10+</a>
 
       <h4 class="week_log">Entry for week<a href="#" data-reveal-id="week1">-1</a><a href="#" data-reveal-id="week2">1</a><a href="#" data-reveal-id="week3">2</a><a href="#" data-reveal-id="week4">3</a><a href="#" data-reveal-id="week5">4</a><a href="#" data-reveal-id="week6">5</a><a href="#" data-reveal-id="week7">6</a><a href="#" data-reveal-id="week8">7</a><a href="#" data-reveal-id="week9">8</a><a href="#" data-reveal-id="week10">9</a><a href="#" data-reveal-id="week11">10</a><a href="#" data-reveal-id="week12">10+</a>
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       <p></p>
 
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       <p>Promoter-recombinase constructs have been successful made and transformed into S. meliloti and MAGE testing is under way.</p>
 
       <p>Promoter-recombinase constructs have been successful made and transformed into S. meliloti and MAGE testing is under way.</p>
       <p class="text-center"><img src="http://client.cameronyick.us/igem/assets/img/journal/pigeon.jpg"></p>
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       <p class="text-center"><img src="https://static.igem.org/mediawiki/2015/thumb/c/c5/Electroporation_of_pKT230_into_R_tropici.jpeg/1600px-Electroporation_of_pKT230_into_R_tropici.jpeg"></p>
 
       <p></p>
 
       <p></p>
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf" class="file__link">Go to the Lab Notebook</a></p>
 
       <p class="text-center"><a href="https://static.igem.org/mediawiki/2015/f/ff/Yale_iGEM_Notebook_2015.pdf" class="file__link">Go to the Lab Notebook</a></p>

Latest revision as of 03:26, 19 September 2015


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