Team:ZJU-China/project s1 1.htm

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Summary

We aimed to design and assemble tunable scaffolds. In order to reach this goal, we utilized the working mechanism of riboswitches. A designed theophylline aptamer was added on the basic RNA scaffold in order to achieve the controllability of it. Since this kind of tunable scaffolds contains an allosteric aptamer, we named them alloscaffolds. The series of alloscaffolds we designed are called ‘clover’. Three versions of clovers were designed, which have different interaction sites and different relative positions between theophylline aptamer and MS2 aptamer as well.

If scaffold library is a disperse scaffold bank, alloscaffold series serves as a successional scaffold bank which includes a variety of scaffolds with diverse efficiencies, realizing by theophylline.

As a preliminary experiment, we use theophylline of different concentrations to test two existing parts, which are riboswitches containing a theophylline aptamer.

Clover version 2 and 3 has been synthesized and characterized. They were respectively co-transformated into E.coli with Fa-MS2 and Fb-PP7 fusion proteins. As a result, in a certain range of theophylline concentration, the fluorescent intensity has a positive correlation with it, which means tunable alloscaffolds are achieved. Compared with clover version 2, version 3 has a better and more stable control effect. Besides, to our surprise, the fluorescent could reach a higher intensity than the basic RNA scaffold, which means our clovers can bring a higher efficiency to pathways.

More work will be done in the future. Except alloscaffold, we are aiming to find new and better methods to design and assemble tunable RNA scaffolds. We believe that more RNA scaffolds with higher efficiency and better regulative effect will be designed and applied in the future.

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 <h2>Summary</h2>
 <p align="justify">&nbsp;</p>
-<p align="justify">On the fundament that RNA scaffold in vivo has been achieved, we aimed to design and assemble controllable scaffolds. A designed theophylline aptamer was added on the original scaffold D0 in order to produce an interaction with MS2 aptamer in the absence of theophylline, thus disturbing the bind of MS2 aptamer and corresponding protein. However in the presence of theophylline, the interaction would disappear with the change of theophylline aptamer. We called these controllable scaffolds 'clovers'. Three versions of clover were designed, which have different interaction sites and different relative positions between the theophylline and MS2 aptamers. </p>
+<p align="justify">We aimed to design and assemble tunable scaffolds. In order to reach this goal, we utilized the <b class="orange">working mechanism of riboswitches. A designed theophylline aptamer</b> was added on the basic RNA scaffold in order to achieve the controllability of it. Since this kind of tunable scaffolds contains <b class="orange">an allosteric aptamer</b>, we named them alloscaffolds. The series of alloscaffolds we designed are called ‘clover’. <b class="orange">Three versions of clovers</b> were designed, which have different interaction sites and different relative positions between theophylline aptamer and MS2 aptamer as well. </p>
+</br>
+<p>If scaffold library is a disperse scaffold bank, alloscaffold series serves as a successional scaffold bank which includes a variety of scaffolds with diverse efficiencies, realizing by theophylline.</p>
 </br>
-<p align="justify">As a preliminary experiment, we use theophylline of different concentrations to test two existing parts, which consist of the gene of a theophylline aptamer and a fluorescent protein. </p>
+<p align="justify">As a preliminary experiment, we use theophylline of different concentrations to <b class="orange">test two existing parts</b>, which are riboswitches containing a theophylline aptamer. </p>
 </br>
-<p align="justify">Clover version two has been synthesized; it was co-transformated into E.coli with Fa-MS2 and Fb-PP7 fusion proteins. As a result, in a certain range of theophylline concentration, the fluorescent intensity has a positive correlation with it, which means controllable scaffold is achieved. Besides, to our surprise, the fluorescent could reach a higher intensity than the original scaffold D0, which means our clover, makes lovers closer!</p>
+<p align="justify">Clover version 2 and 3 has been synthesized and characterized.  They were respectively co-transformated into <i>E.coli</i> with Fa-MS2 and Fb-PP7 fusion proteins. As a result, in a certain range of theophylline concentration, the fluorescent intensity has a positive correlation with it, which means <b class="orange">tunable alloscaffolds are achieved</b>. Compared with clover version 2, version 3 has a better and more stable control effect. Besides, to our surprise, the fluorescent could reach a higher intensity than the basic RNA scaffold, which means our clovers can <b class="orange">bring a higher efficiency to pathways</b>.</p>
 </br>
-<p align="justify">More future work will be done in the next period. We are going to synthesize clover version one and version three, which seem to have a better control effect. A comparison will be made to find the best design principle of controllable RNA scaffold. We believe that more RNA scaffolds with higher efficiency and better regulative effect will be designed and applied.</p>
+<p align="justify">More work will be done in the future. Except alloscaffold, we are aiming to <b class="orange">find new and better methods to design and assemble tunable RNA scaffolds</b>. We believe that more RNA scaffolds with higher efficiency and better regulative effect will be designed and applied in the future. </p>
 </br>
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