Difference between revisions of "Team:MSU-Michigan/Parts"

 
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<h1>Parts</h1>
 
<h1>Parts</h1>
  
  
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<h5>Adding parts to the registry</h5>
 
<p>You can add parts to the Registry at our <a href="http://parts.igem.org/Add_a_Part_to_the_Registry">Add a Part to the Registry</a> link.</p>
 
  
  
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<h5>What information do I need to start putting my parts on the Registry?</h5>
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<p>The parts were taken from the Shewanella oneidensis MR-1 genome by finding a regulator on <a href="http://regprecise.lbl.gov/RegPrecise/">RegPrecise.</a> Then the consensus sequence was located at the appropriate distance from a gene and DNA upstream from the gene was taken, which included the consensus sequence.  This ensured that the ribosomal binding site would be in the sequence we took as well as any other necessary machinery for the following gene to be regulated by the promoter that we extracted.  All of the promoters were then amplified using PCR and inserted into the prL814 plasmid in place of the T7A1 promoter.
<p>The information needed to initially create a part on the Registry is:</p>
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<ul>
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<li>Part Name</li>
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<li>Part type</li>
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<li>Creator</li>
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<li>Sequence</li>
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<li>Short Description (60 characters on what the DNA does)</li>
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<li>Long Description (Longer description of what the DNA does)</li>
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<li>Design considerations</li>
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Each part that the MSU iGEM team constructed, was taken from the Shewanella oneidensis MR-1 genome by finding a regulator for each desired part on http://regprecise.lbl.gov/RegPrecise/. These parts were all built to detect contaminants. A provided consensus sequence was then taken at the appropriate distance from a gene and included with the DNA that is upstream from that gene. This selection process ensured that the ribosomal binding site would be in the sequence taken, as well as any other necessary machinery for the following gene to be regulated by the promoter that was extracted. All of the promoters were then amplified using PCR and inserted into the prL814 plasmid in place of the T7A1 promoter. From the nine parts created ( part numbers listed below) Paraquat was the main part that the MSU team chose to pursue for GFP experiments, and proof of concept, due to no metabolic relevance to the cell.
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<p>The parts were taken from the Shewanella oneidensis MR-1 genome by finding a regulator on http://regprecise.lbl.gov/RegPrecise/.  Then taking the consensus sequence provided at the appropriate distance from a gene and taking the DNA that is upstream from the gene including the consensus sequence.  This ensured that the ribosomal binding site would be in the sequence we took as well as any other necessary machinery for the following gene to be regulated by the promoter that we extracted.  All of the promoters were then amplified using PCR and inserted into the prL814 plasmid in place of the T7A1 promoter.</p>
 
  
  
 
<h2>Part Table </h2>
 
<h2>Part Table </h2>
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<groupparts>iGEM17 MSU-Michigan</groupparts>
 
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{{MSU-Michigan-Footer}}

Latest revision as of 03:24, 2 November 2017

Parts

The parts were taken from the Shewanella oneidensis MR-1 genome by finding a regulator on RegPrecise. Then the consensus sequence was located at the appropriate distance from a gene and DNA upstream from the gene was taken, which included the consensus sequence. This ensured that the ribosomal binding site would be in the sequence we took as well as any other necessary machinery for the following gene to be regulated by the promoter that we extracted. All of the promoters were then amplified using PCR and inserted into the prL814 plasmid in place of the T7A1 promoter.

Each part that the MSU iGEM team constructed, was taken from the Shewanella oneidensis MR-1 genome by finding a regulator for each desired part on http://regprecise.lbl.gov/RegPrecise/. These parts were all built to detect contaminants. A provided consensus sequence was then taken at the appropriate distance from a gene and included with the DNA that is upstream from that gene. This selection process ensured that the ribosomal binding site would be in the sequence taken, as well as any other necessary machinery for the following gene to be regulated by the promoter that was extracted. All of the promoters were then amplified using PCR and inserted into the prL814 plasmid in place of the T7A1 promoter. From the nine parts created ( part numbers listed below) Paraquat was the main part that the MSU team chose to pursue for GFP experiments, and proof of concept, due to no metabolic relevance to the cell.

Part Table

Biobricks

"Confirmation of promoters induced by (from left to right) Blue light, Paraquat, Nitrate (NO3), and Copper"

<groupparts>iGEM17 MSU-Michigan</groupparts>

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