Difference between revisions of "Team:Warwick/Modelling2"

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<br>As you can see from the images above to accomplish this we will cut correct lengths of DNA out of already available plasmid inserts then denature them, binding two single stranded pieces of DNA together to form a string of twice the length. Doing this allows origami to be used to form a structure as the sides of the single strands will have a complementary pair. This also allows for quick PCR.
 
<br>As you can see from the images above to accomplish this we will cut correct lengths of DNA out of already available plasmid inserts then denature them, binding two single stranded pieces of DNA together to form a string of twice the length. Doing this allows origami to be used to form a structure as the sides of the single strands will have a complementary pair. This also allows for quick PCR.
 
<br>We decided to use plasmids from the last two years iGEM part registry.
 
<br>We decided to use plasmids from the last two years iGEM part registry.
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<p>Below shows the process by which the DNA origami structures are made using already available DNA.</p><br><br>
  
 
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Revision as of 17:57, 16 September 2015

Warwick iGEM 2015