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Team:Freiburg/Highlights
From 2013.igem.org
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<li>...design a <b>catalytically inactive version of Cas9</b> and designing a new class of DNA binding proteins.</li> | <li>...design a <b>catalytically inactive version of Cas9</b> and designing a new class of DNA binding proteins.</li> | ||
| - | <li>...combine this modified | + | <li>...combine this modified dCas9 with <b>different effectors</b>.</li> |
<li>...express the system in various <b>mammalian cell lines</b>.</li> | <li>...express the system in various <b>mammalian cell lines</b>.</li> | ||
<li>...control human <b>gene expression</b> via our modified CRISPR/Cas system.</li> | <li>...control human <b>gene expression</b> via our modified CRISPR/Cas system.</li> | ||
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</p> | </p> | ||
<p> | <p> | ||
| - | A mutated Cas9 derived protein without nickase function was our start. This is basically a DNA binding protein, that is relying on a <b>protein-RNA-DNA </b> | + | A mutated Cas9 derived protein without nickase function was our start. This is basically a DNA binding protein, that is relying on a <b>protein-RNA-DNA</b> |
| - | + | ||
interaction. | interaction. | ||
</p><p></p><p> | </p><p></p><p> | ||
| - | By fusing <b>effector domains</b> to | + | By fusing <b>effector domains</b> to dCas9 we altered the properties in various ways.</p> |
<p id="h3">Activation | <p id="h3">Activation | ||
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<tr> | <tr> | ||
<td> <b>Figure 1: Activation by Cas9:VP16 </b><br> | <td> <b>Figure 1: Activation by Cas9:VP16 </b><br> | ||
| - | By fusing the transcriptional activation domain VP16 to | + | By fusing the transcriptional activation domain VP16 to dCas9, we are able to activate a SEAP reporter transcription. |
</td> | </td> | ||
</tr> | </tr> | ||
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</div> | </div> | ||
| - | <p id="h3">Repression | + | <p id="h3"> Repression |
</p> | </p> | ||
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</tr> | </tr> | ||
<tr> | <tr> | ||
| - | <td> <b>Figure 2: Repression via | + | <td> <b>Figure 2: Repression via dCas9:KRAB </b><br> |
| - | Using | + | Using dCas9:KRAB we were able to repress GFP expression in mammalian cells. |
</td> | </td> | ||
</tr> | </tr> | ||
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</tr> | </tr> | ||
<tr> | <tr> | ||
| - | <td> <b>Figure 3: Endogenous, stable repression by | + | <td> <b>Figure 3: Endogenous, stable repression by dCas9:G9a </b><br> |
| - | Chromatin remodeling, resulting in repression of endogenous genes is possible by fusing the histone methyltransferase G9a to | + | Chromatin remodeling, resulting in repression of endogenous genes is possible by fusing the histone methyltransferase G9a to dCas9. |
</td> | </td> | ||
</tr> | </tr> | ||
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We developed an ELISA based method. With this method we can quantify the <b>binding efficiency </b>of our proteins. We called this binding assay <b>uniBAss</b>. It is | We developed an ELISA based method. With this method we can quantify the <b>binding efficiency </b>of our proteins. We called this binding assay <b>uniBAss</b>. It is | ||
| - | a powerful tool for the characterization of the interaction between the modified | + | a powerful tool for the characterization of the interaction between the modified dCas9 and the locus specific RNA. |
</p> <p> | </p> <p> | ||
<div> | <div> | ||
Revision as of 20:53, 29 September 2013
Highlights
In the last months we were able to...
- ...design a catalytically inactive version of Cas9 and designing a new class of DNA binding proteins.
- ...combine this modified dCas9 with different effectors.
- ...express the system in various mammalian cell lines.
- ...control human gene expression via our modified CRISPR/Cas system.
- ...control gene expression on light stimulus.
- ...standardize dCas9 by mutating illegal iGEM restriction sites.
Our toolkit ...
A mutated Cas9 derived protein without nickase function was our start. This is basically a DNA binding protein, that is relying on a protein-RNA-DNA interaction.
By fusing effector domains to dCas9 we altered the properties in various ways.
Activation
The activation domain VP16 is able to activate transcription of genes.
 |
| Figure 1: Activation by Cas9:VP16 By fusing the transcriptional activation domain VP16 to dCas9, we are able to activate a SEAP reporter transcription. |
Repression
The fusion of the transcriptional repressor domain KRAB leads to synthetic repression of gene expression.  |
| Figure 2: Repression via dCas9:KRAB Using dCas9:KRAB we were able to repress GFP expression in mammalian cells. |
Chromatin modification (Repression)
Specific chromatin modification was achieved by fusing a histone methyltransferase G9a to dCas9. With this protein we are able to specifically repress endogenous gene expression.
 |
| Figure 3: Endogenous, stable repression by dCas9:G9a Chromatin remodeling, resulting in repression of endogenous genes is possible by fusing the histone methyltransferase G9a to dCas9. |
Light switch
We were able to induce our system on light stimulus. This was possible by using photorecetors of higher plants.
Targeting with RNAimer
By building a plasmid containing the necessary RNAs and insertion sites for targeting we created a modular, BioBrick compatible system for multiple DNA targeting: The RNAimer. Using our RNAimer plasmid it is easy to combine several target sequences on one plasmid using the BioBrick standard.
uniBAss - Binding Assay
We developed an ELISA based method. With this method we can quantify the binding efficiency of our proteins. We called this binding assay uniBAss. It is a powerful tool for the characterization of the interaction between the modified dCas9 and the locus specific RNA.
 |
| Figure 4: uniBAss We developed an assay for testing the binding capacity of our constructs. |
Conclusion
In summary, we established a new modularized toolkit for modulating gene expression: The uniCAS Toolkit!
