Difference between revisions of "Team:Pittsburgh/Notebook"

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{{Pittsburgh}}
 
{{Pittsburgh}}
 
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<span class="anchor" id="Week1"></span>
 
<span class="anchor" id="Week1"></span>
 
<h1>Week 1: May 23 - May 27</h1>
 
<h1>Week 1: May 23 - May 27</h1>
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<img src="https://static.igem.org/mediawiki/2016/b/b8/T--Pittsburgh--NotebookWetLab.jpg" alt="Wet Lab" style="padding:5px; width:100px;height:100px;float:left;">
<tr><td><img style="padding:5px;width:100px;height:100px;" src="https://static.igem.org/mediawiki/2016/b/b8/T--Pittsburgh--NotebookWetLab.jpg" alt="Wet Lab"></td>
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<td><ul>
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<ul style="padding:5px; display:block; float:left; ">
 
<li>Training begins</li>
 
<li>Training begins</li>
 
<li>Grow Top 10 <a href="https://2016.igem.org/Team:Pittsburgh/Protocols#competent" target="_blank">competent cells</a>.</li>
 
<li>Grow Top 10 <a href="https://2016.igem.org/Team:Pittsburgh/Protocols#competent" target="_blank">competent cells</a>.</li>
 
</ul>
 
</ul>
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<h2>Dry Lab</h2>
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<td><img style="padding:5px;width:100px;height:100px;" src="https://static.igem.org/mediawiki/2016/e/e0/T--Pittsburgh--NotebookDryLab.jpg" alt="Dry Lab"></td>
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    <td>
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<ul>
 
<ul>
 
<li>Brainstorm genetic circuits for a thallium sensor</li>
 
<li>Brainstorm genetic circuits for a thallium sensor</li>
 
<li>Lab safety training</li>
 
<li>Lab safety training</li>
 
</ul>
 
</ul>
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</table>
 
 
<a href=https://static.igem.org/mediawiki/2016/b/bc/TeamPittsburghNotebookWeek1.pdf target="_blank">Week 1 Notebook</a><br>
 
<a href=https://static.igem.org/mediawiki/2016/b/bc/TeamPittsburghNotebookWeek1.pdf target="_blank">Week 1 Notebook</a><br>
 
<a href="#Top">Back to Top</a>
 
<a href="#Top">Back to Top</a>

Revision as of 20:41, 30 July 2016

Our weekly progress. For a list of our protocols, visit the Protocols page

Week 1: May 23 - May 27

Wet Lab

Dry Lab

  • Brainstorm genetic circuits for a thallium sensor
  • Lab safety training
Week 1 Notebook
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Week 2: May 31 - June 3

Wet Lab

Cell-Free Extract

Dry Lab

  • Contact museums and summer programs for outreach opportunities
  • Lab safety training
Week 2 Notebook
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Week 3: June 6 - June 12

Wet Lab

Reporter

  • Transform T7 promoter, amilCP, and terminator
  • Begin assembly by ligating linearized T7 promoter and amilCP

Dry Lab

  • Contact museums and summer programs for outreach opportunities
Week 3 Notebook
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Week 4: June 13 - June 17

Wet Lab

Reporter

  • Transform T7-GFP plasmid, lacZ alpha fragment, and eGFP
  • Send promising T7 promoter -- amilCP ligations to be sequenced
  • Perform double digest of T7 promoter and terminator from last week
  • Ligate double-digested T7 promoter to new reporters (lacZ and eGFP)

Dry Lab

  • TECBio, DiSCoBio, and Tissue Engineering Camp outreach opportunities set
Week 4 Notebook
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Week 5: June 20 - June 26

Wet Lab

Cell-Free Extract

  • Reaction volume can be reduced to 5 μL with 5 ng/μL of DNA

Toehold Switch

  • Collins triggers activate the switches (both in plasmid form) to express LacZ

Reporter

  • Ligate T7 promoter -- amilCP construct to terminator
  • Extract successful ligations of T7 promoter to eGFP
  • Ligate T7 promoter -- eGFP construct to terminator

Dry Lab

  • Reach out to teams to collaborate based on last year's projects
Week 5 Notebook
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Week 6: June 27 - July 3

Wet Lab

Cell-Free Extract

  • Reaction volume can be reduced to 1 μL with 5 ng/μL of DNA

Toehold Switch

  • Collins plasmids express LacZ with 25 ng of switch
  • DNA oligos trigger Collins switches

Reporter

  • Identify successful ligations to terminator for amilCP and eGFP consturcts using a gel
  • Send correct plasmids for sequencing for confirmation
  • Test plasmids in cell-free extract
  • amilCP does not produce color in cell-free reaction
  • eGFP produces fluorescence comparable to that from the Collins T7-GFP plasmid in cell-free reaction
  • Linearized plasmids containing only the promoter and insert (no terminator) do not express protein

Dry Lab

  • Work on outreach presentation for tissue engineering camp
Week 6 Notebook
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Week 7: July 5 - July 8

Wet Lab

Cell-Free Extract

  • 384-well plate requires at least 10 μL of reaction

DNAzyme

  • Anneal PO strand with catalytic strand, both with and without erbium
  • Test success of annealing reaction in cell-free extract and with acrylamide gels

Reporter

  • Sequenced amilCP construct does not contain amilCP
  • Unsuccessfully linearize and amplify eGFP construct using PCR

Dry Lab

  • Practice outreach presentation for tissue engineering camp
  • Develop DNAzymes for other heavy metals
Week 7 Notebook
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Week 8: July 11 - July 17

Wet Lab

Cell-Free Extract

  • Linear eGFP construct does not produce a stronger signal than its plasmid form

DNAzyme

  • DNAzyme duplex does not trigger toehold switch
  • Erbium cleaves the P substrate strand

Reporter

  • Restart amilCP cloning process

Dry Lab

  • First presentation at Camp BioE
  • Prepare for UMD Mid-Atlantic Meet-Up
  • Contact PLSG and NEB for sponsorship
Week 8 Notebook
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Week 9: July 18 - July 22

Wet Lab

Cell-Free Extract

  • Reactions can be diluted by one-half and still produce visible results in two hours

DNAzyme

  • dPAGE assay of P substrate cleavage suggests that the DNAzyme works, but results are not definitive
  • Six-hour time course of cleavage does not yield much additional information
  • Reaction temperature (room temperature versus 37°C) does not produce observable effect on cleavage rates

Reporter

  • Continue amilCP cloning process
  • Clone RBS-T3 RNA polymerase to add into other constructs

Dry Lab

  • Presentation at Camp BioE
  • UMD Mid-Atlantic Meet-Up
  • Continue fundraising
  • Discuss systems to model
Week 9 Notebook
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