Difference between revisions of "Team:William and Mary/Interlab Study"

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                     <p class="h2WM">Interlab Study</p>
 
                     <p class="h2WM">Interlab Study</p>
 
                     <p class="description"></p>
 
                     <p class="description"></p>
<p>We participated in the Interlab Measurement Study! We created are fluorescent constructs using DNA synthesis and Gibson Assembly. The constructs we measured were J23101 + I13504, J23106 + I13504, and J23117 + I13504.  
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<p>We created our fluorescent constructs using DNA synthesis and Gibson Assembly. The constructs we measured were J23101 + I13504, J23106 + I13504, and J23117 + I13504.  
 
We assembled the gBlocks using our <a href = "https://2015.igem.org/Team:William_and_Mary/Protocols:Gibson">Gibson assembly protocol</a>, and imaged the constructs using our <a href = "https://2015.igem.org/Team:William_and_Mary/Protocols:Imaging">imaging protocol</a>.</p>
 
We assembled the gBlocks using our <a href = "https://2015.igem.org/Team:William_and_Mary/Protocols:Gibson">Gibson assembly protocol</a>, and imaged the constructs using our <a href = "https://2015.igem.org/Team:William_and_Mary/Protocols:Imaging">imaging protocol</a>.</p>
 
<p> Cells were identified using Nikon Elements Software version 7.1 using binary thresholding on the GFP channel. Nikon Elements Software was then used to calculate mean fluorescence per cell and data was exported to Excel for final data analysis.  </p>
 
<p> Cells were identified using Nikon Elements Software version 7.1 using binary thresholding on the GFP channel. Nikon Elements Software was then used to calculate mean fluorescence per cell and data was exported to Excel for final data analysis.  </p>

Revision as of 23:28, 18 September 2015

NOISE - W&M iGEM

Interlab Study

We created our fluorescent constructs using DNA synthesis and Gibson Assembly. The constructs we measured were J23101 + I13504, J23106 + I13504, and J23117 + I13504. We assembled the gBlocks using our Gibson assembly protocol, and imaged the constructs using our imaging protocol.

Cells were identified using Nikon Elements Software version 7.1 using binary thresholding on the GFP channel. Nikon Elements Software was then used to calculate mean fluorescence per cell and data was exported to Excel for final data analysis.

Our data are shown below: