Difference between revisions of "Team:Austin LASA/Design"

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     p('We planned to do so by designing circuits to express Bst and LbCas12a enzymes in bacteria. This bacteria would be grown, induced to produce enzyme, after which the bacteria would be lyophilized. Unfortunately, we were unable to get to this step. However, we did design potential circuits to be used in cellular reagents.'),
 
     p('We planned to do so by designing circuits to express Bst and LbCas12a enzymes in bacteria. This bacteria would be grown, induced to produce enzyme, after which the bacteria would be lyophilized. Unfortunately, we were unable to get to this step. However, we did design potential circuits to be used in cellular reagents.'),
 
     p('(See our Experiments page for more information on how to create cellular reagents).')
 
     p('(See our Experiments page for more information on how to create cellular reagents).')
 +
  ),
 +
  h(g.Section, {title: 'LAMP Cellular Reagents'},
 +
    p('Our lab has already developed LAMP cellular reagents. Therefore, we were advised by our supervisors to focus on developing Cas12a cellular reagents.')
 +
  ),
 +
  h(g.Section, {title: 'Cas12a Cellular Reagents'},
 +
    p('We designed Cas12a gene circuits that expressed LbCas12a and a corresponding crRNA. We did not have time to clone these circuits, but we did include them in our parts collection.'),
 +
    p('Each circuit contains a transcriptional unit which expressed LbCas12a. Adjacent and in the opposite direction is a transcriptional unit coding for a crRNA. Unfortunately, we did not have the time to clone these circuits and create cellular reagents.')
 +
  ),
 +
  h(g.Section, {title: 'In the end, what did we do?',
 +
    p('We were able to detect our viral DNA with four different specifically designed crRNA sequences with purified enzyme.'),
 +
    p('We were able to amplify regions of our viral DNA (Rev) with four different LAMP primer sets with purified enzyme.'),
 +
    p('We did not have the time to detect our LAMP amplicons with our Cas12a assay.'),
 +
    p('We did not have the time to create cellular reagents with which to test our LAMP and Cas12a reactions.')
 
   )
 
   )
 
);
 
);
 
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Revision as of 02:46, 18 October 2018