Difference between revisions of "Team:Bielefeld-CeBiTec/Description"

 
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<h1 style="margin-bottom: 0px; text-align:left">Project Description</h1>
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<h2 style="color:#ffffff; text-align:left">The only way to do great work is to love what you do - Steve Jobs</h2>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description">Description</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation">Mutation</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Fermentation">Fermentation</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Collaborations/Freiburg">Freiburg</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Experiments/Primers">Primers</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Team">Official Team Profile</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Team/Bielefeld_University">University Bielefeld</a></li>
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<li><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Acknowledgement">Overview</a></li>
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<div class="container main">
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<div class="container text_header"><h1>Project description</h1></div>
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<div class="container text_header"><h3>Fast evolving pathogens as global health threat</h3></div>
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<div class="container text">
 
<div class="container text">
coming soon...
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            As long as mankind remembers, different diseases struck from time to time and demanded millions of lives.  
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            Maybe the most fatal of these epidemic outbreaks was the 1918 flu pandemic, which killed between 50-100 million people worldwide.
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            Derived from a simple influenza virus only a few mutations were necessary to change this virus into one of the deadliest threats
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            that ever existed. Pandemic viral infections like this were the reason for our project selection. Our highest
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            motivation was to create a system to counteract these
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            extremely high risk potential slumbering in commonly known and seemingly not to dangerous viruses. Of course the influenza virus
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            stated 1918 a much higher risk than it does today. But still viruses are very hard to treat and especially members of the family <i>flaviviridae</i>
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            like Zika or Dengue virus, show a high risk potential because of their high mutation rate.
 +
            <br>We found a way to create in a short period of time antibody-like proteins.
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            Evobodies are binding
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            proteins that are able to be quickly adapted to altered targets like viral hull proteins and
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            re-establish binding properties in extremely short periods of time
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            The limiting factors in this process are the rate at which mutations happen in the gene of the Evobody
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            and screening of different proteins. This is the reason why we wanted to build a mutation inducing system
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            which is not only able to change basepairs <i>in vivo</i> at a very high frequency,
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            but is also specific enough to provide stability in culture
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            and does not interfere too much with growth properties of the individual cell.
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        </div>
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        <div class="container text">
 +
       
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            The revolutionary part of Evobody generation is the combination of an <i>in vivo</i> mutagenesis
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            and a selection system which is also capable of screening our mutants during the process of
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            cell cultivation. Due to our constant interaction of altered binding proteins and the <i>in vivo</i>
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            selection, we were eager to increase the mutation rate while retaining normal growth conditions. That is
 +
            why we did not only calculate the mutation rate of our two different mutagenesis approaches,
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            but also determined the growth rate under
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            different conditions.
 +
       
 
</div>
 
</div>
 
<div class="container text_header"><h3>Generation of binding proteins by directed evolution</h3></div>
 
<div class="container text_header"><h3>Generation of binding proteins by directed evolution</h3></div>
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This year the iGEM Team Bielefeld-CeBiTec aims to create a method for generating synthetic binding proteins,  
 
This year the iGEM Team Bielefeld-CeBiTec aims to create a method for generating synthetic binding proteins,  
 
our so-called Evobodies. This works by creating a library of binding proteins and increasing their affinity  
 
our so-called Evobodies. This works by creating a library of binding proteins and increasing their affinity  
towards a target by directed evolution (Fig. 1). As a starting point, we randomise the binding regions of  
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towards a target by directed evolution (Figure 1). As a starting point, we randomize the binding regions of  
synthetic antibody-like proteins (Fig. 1a). Following we screen this library for affinity towards a target by  
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synthetic antibody-like proteins (Figure 1A). Following we screen this library for affinity towards a target by  
using a bacterial two-hybrid system (Fig. 1b). To further increase the Evobodies affinity, we combine the selection  
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using a bacterial two-hybrid system (Figure 1B). To further increase the Evobodies affinity, we combine the selection  
via the two-hybrid system with an <i>in vivo</i> mutagenesis system (Fig. 1c). Doing this we hope to generate strong  
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via the two-hybrid system with an <i>in vivo</i> mutagenesis system (Figure 1C). Doing this we hope to generate strong  
and specific binding proteins by combining the powerful genetics of <i>E. coli</i> with the biological idea of  
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and specific binding proteins by combining the powerful genetics of <i>E.&nbsp;coli</i> with the biological idea of  
 
antibody generation and maturation in vertebrates.
 
antibody generation and maturation in vertebrates.
<br>
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<center><figure class="figure">
<div class="image_description">
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<img src="https://static.igem.org/mediawiki/2016/b/b9/Bielefeld_CeBiTec_2016_10_19_XXXX_Overview_project_desc.png" class="figure-img" />
<b>Figure 1: Overview</b>
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<figcaption class="figure-caption">
</div>
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<b>Figure 1: Schematic Evobody generation process</b>. A library of synthetic binding proteins (A) is screened by a bacterial two hybrid(B) for interaction with a traget protein. Existing interaction between both proteins leads to expression of a resistance gene thus granting the individual cell a selection advantage. After screening the library all suviving clones binding proteins are mutagenized <i>in vivo</i> (C) which results in the generation of new binding properties. Continuous selection cycles of selection and mutation increase the Evobodies binding affinity towards high affine binding proteins. 
<br><br>
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</figcaption>
 +
</figure></center>
 
We designed our Evobody approach as an alternative to conventional methods for the generation of binding proteins.  
 
We designed our Evobody approach as an alternative to conventional methods for the generation of binding proteins.  
 
In our vision it should be possible to clone each protein encoding sequence into one of our plasmids, let our system  
 
In our vision it should be possible to clone each protein encoding sequence into one of our plasmids, let our system  
Line 423: Line 73:
 
We identified amino acids, which are present in most protein-protein interaction areas and created a randomization  
 
We identified amino acids, which are present in most protein-protein interaction areas and created a randomization  
 
scheme so that only these amino acids are encoded in the antibody-mimetics binding region. Read more about our  
 
scheme so that only these amino acids are encoded in the antibody-mimetics binding region. Read more about our  
library design <a href=”https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Library”>here</a>.
+
library design <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Library">here</a>.<br><br>
 
+
<center><figure class="figure">
<br>
+
<img src="https://static.igem.org/mediawiki/2016/f/fd/Bielefeld_CeBiTec_2016_10_19_LIB_general_binding_proteins_overview_with_chimera.png" width=60% class="figure-img" /><br><br>
<div class="image_description">
+
<figcaption class="figure-caption">
<b>Figure 2: Library</b>
+
<b>Figure 2: Library of initial binding proteins.</b> Expression of the initial binding proteins with variable regions highlighted in seperate colors (turquoise, orange, white, green, pink and blue) and constant regions in olive. The theoretical variability for each scaffold is 1.073.741.824.
</div>
+
</figcaption>
 +
</figure></center>
 
</div>
 
</div>
 
<div class="container text_header"><h3>Survival of the fittest - bacterial two-hybrid</h3></div>
 
<div class="container text_header"><h3>Survival of the fittest - bacterial two-hybrid</h3></div>
 
<div class="container text">
 
<div class="container text">
 
In the next step, the binding protein library should be screened for proteins with an innate affinity for our target.  
 
In the next step, the binding protein library should be screened for proteins with an innate affinity for our target.  
We want to realize this by using a bacterial two-hybrid system. Therefore, our target protein (1) is fused to a DNA  
+
We want to realize this by using a bacterial two-hybrid system (Figure 3). Therefore, our target protein (1) is fused to a DNA  
 
binding domain (2), which localises upstream of a reporter cassette (3). The binding protein (4) is fused to a RNA polymerase  
 
binding domain (2), which localises upstream of a reporter cassette (3). The binding protein (4) is fused to a RNA polymerase  
 
subunit (5). Interaction between the binding and the target protein leads to recruitment of the RNA polymerase to the promoter  
 
subunit (5). Interaction between the binding and the target protein leads to recruitment of the RNA polymerase to the promoter  
 
region of the reporter cassette and activates the reporter gene expression. By using an antibiotic resistance as a reporter  
 
region of the reporter cassette and activates the reporter gene expression. By using an antibiotic resistance as a reporter  
gene the output of the  bacterial two hybrid system should lead to the survival <i>E. coli</i> cells carrying a good binding  
+
gene the output of the  bacterial two hybrid system should lead to the survival <i>E.&nbsp;coli</i> cells carrying a good binding  
 
protein and the death of all cells with a bad binding protein.
 
protein and the death of all cells with a bad binding protein.
<center><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Selection"><img src="https://static.igem.org/mediawiki/2016/9/9e/Bielefeld_CeBiTec_2016_10_14_project_description_selection.png" width=60% /></a></center>
+
<center><figure class="figure">
<div class="image_description">
+
<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Selection">
<b>Figure 3: Bacterial-two hybrid system.</b> Interaction between the binding protein (4) and the target protein (1)  
+
<img src="https://static.igem.org/mediawiki/2016/9/9e/Bielefeld_CeBiTec_2016_10_14_project_description_selection.png" width=60% class="figure-img"/>
lead to recruitment of RNA polymerase (5) to the promoter upstream of the reporter cassette (3) and subsequent  
+
</a>
expression of the reporter gene. In this case the reporter is beta-lactamase, which expression leads to degradation  
+
<figcaption class="figure-caption">
of ampicillin (blue squares) and survival of the bacteria.
+
<b>Figure 3: Bacterial-two hybrid system.</b>Interaction between the binding protein (4) and the target protein (1)  
</div>
+
lead to recruitment of RNA polymerase (5) to the promoter upstream of the reporter cassette (3) and subsequent  
<br>
+
expression of the reporter gene. In this case the reporter is beta-lactamase, which expression leads to degradation  
 +
of ampicillin (blue squares) and survival of the bacteria.
 +
</figcaption>
 +
</figure></center>
 
From the two-hybrid system we expect foremost a selection of the binding protein library. Furthermore, we expect a correlation  
 
From the two-hybrid system we expect foremost a selection of the binding protein library. Furthermore, we expect a correlation  
 
between binding - target protein affinity and the activated gene expression strength of the reporter. By using an antibiotic  
 
between binding - target protein affinity and the activated gene expression strength of the reporter. By using an antibiotic  
Line 453: Line 107:
 
which should lead to a higher growth rate under strong selective pressure. The complete two-hybrid system should cumulate in a  
 
which should lead to a higher growth rate under strong selective pressure. The complete two-hybrid system should cumulate in a  
 
correlation between binding protein affinity and bacterial growth rate, which should lead to selection of a few bacteria with  
 
correlation between binding protein affinity and bacterial growth rate, which should lead to selection of a few bacteria with  
strong binding proteins. Find out more on our <a href=” https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Selection“>selection page</a>.
+
strong binding proteins. Find out more on our <a href=” https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Selection“>selection subpage</a>.
</div>
+
</div>
 
<div class="container text_header"><h3>Accessing the sequence space - <i>in vivo</i> mutagenesis</h3></div>
 
<div class="container text_header"><h3>Accessing the sequence space - <i>in vivo</i> mutagenesis</h3></div>
 
<div class="container text">
 
<div class="container text">
 
After selection of the bulk of our library we will increase the affinity of our Evobodies in a process similar to the affinity  
 
After selection of the bulk of our library we will increase the affinity of our Evobodies in a process similar to the affinity  
maturation of antibodies<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Teng2007">(Teng und Papavasiliou 2007)</a>. As  
+
maturation of antibodies (<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Teng2007">Teng und Papavasiliou 2007</a>). As  
 
addressed above we will select our Evobodies by increasing the selection pressure. At the same time, we will use an <i>in vivo</i>  
 
addressed above we will select our Evobodies by increasing the selection pressure. At the same time, we will use an <i>in vivo</i>  
 
mutagenesis system. Thereby ,we can increase the sequence diversity beyond the limits of our library. Slightly modifications of   
 
mutagenesis system. Thereby ,we can increase the sequence diversity beyond the limits of our library. Slightly modifications of   
 
binding proteins identified during the initial selection will are the basis for the directed  evolution.
 
binding proteins identified during the initial selection will are the basis for the directed  evolution.
<center><a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation"><img src="https://static.igem.org/mediawiki/2016/d/d4/Bielefeld_CeBiTec_2016_10_14_project_description_mutation.png" width=60% /></a></center>
+
<center><figure class="figure">
<div class="image_description">
+
<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation">
<b>Figure 4: <i>In vivo</i> mutagenesis system.</b> By using an <i>in vivo</i> mutagenesis system a single Evobody coding  
+
<img src="https://static.igem.org/mediawiki/2016/d/d4/Bielefeld_CeBiTec_2016_10_14_project_description_mutation.png" width=60% class="figure-img"/>
sequence can be evolved to various different variants, each with a unique binding site. The single starting sequence is  
+
</a>
replicated during growth and thereby mutations are incorporated either through error-prone polymerase I or a combination  
+
<figcaption class="figure-caption">
of global mutator genes. The process results in the creating of the library of binding proteins with different binding properties.
+
<b>Figure 4: <i>In vivo</i> mutagenesis system.</b> By using an <i>in vivo</i> mutagenesis system a single Evobody coding  
</div>
+
sequence can be evolved to various different variants, each with a unique binding site. The single starting sequence is  
 +
replicated during growth and thereby mutations are incorporated either through error-prone polymerase I or a combination  
 +
of global mutator genes. The process results in the creating of the library of binding proteins with different binding properties.
 +
</figcaption>
 +
</figure>
 +
</center>
 
<br>
 
<br>
 
In detail, we will compare two different possibilities to diversify our binding proteins. The first approach is the use of an  
 
In detail, we will compare two different possibilities to diversify our binding proteins. The first approach is the use of an  
error-prone polymerase I in an otherwise Pol I temperature-sensitive <i>E. coli</i> strain. <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">(Camps et al. 2003)</a>  
+
error-prone polymerase I in an otherwise Pol I temperature-sensitive <i>E.&nbsp;coli</i> strain.  
 +
(<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">Camps et al. 2003</a>)
 
Growth at a non-permissive temperature should result in accumulation of mutations in the part of the genom maintained by DNA polymerase I.  
 
Growth at a non-permissive temperature should result in accumulation of mutations in the part of the genom maintained by DNA polymerase I.  
 
The interesting idea behind this approach is the fact that large parts of plasmids carrying an origin of replication from the  
 
The interesting idea behind this approach is the fact that large parts of plasmids carrying an origin of replication from the  
ColE1-familiy are replicated by the polymerase I. <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">(Camps et al. 2003;</a> <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2010">Camps 2010)</a>  
+
ColE1-familiy are replicated by the polymerase I. (<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">Camps et al. 2003</a>; <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2010">Camps 2010</a>)
 
Because of this, the usage of the error-prone polymerase I should mutant mainly our Evobody sequence on a plasmid. Thereby off-target  
 
Because of this, the usage of the error-prone polymerase I should mutant mainly our Evobody sequence on a plasmid. Thereby off-target  
mutations, which are a major obstacle of <i>in vivo</i> mutagenesis, should be minimized. <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">(Camps et al. 2003)</a><br>
+
mutations, which are a major obstacle of <i>in vivo</i> mutagenesis, should be minimized. (<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Camps2003">Camps et al. 2003</a>)<br>
Our other approach is based on creating a plasmid borne hypermutator system by modulating the <i>E. coli</i> DNA fidelity systems.  
+
Our other approach is based on creating a plasmid borne hypermutator system by modulating the <i>E.&nbsp;coli</i> DNA fidelity systems.  
<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Badran2015">(Badran und Liu 2015)</a> We will express known mutator genes under tight regulation from a plasmid. By using a plasmid borne mutator  
+
(<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Badran2015">Badran und Liu 2015</a>) We will express known mutator genes under tight regulation from a plasmid. By using a plasmid borne mutator  
 
system, in contrast to the more classical approaches of incorporating the mutator genes directly inside the genom.  
 
system, in contrast to the more classical approaches of incorporating the mutator genes directly inside the genom.  
<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#AgilentTech">(Agilent Technologies;</a> <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Greener1997">Greener et al. 1997)</a>  Thereby we want to circumvent the known problems with globally increased mutation rate,  
+
(<a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#AgilentTech">Agilent Technologies</a>; <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Description#Greener1997">Greener et al. 1997</a>)  
which are genetic instability or general unviability.<br>
+
Thereby we want to circumvent the known problems with globally increased mutation rate, which are genetic instability or general unviability.<br>
 
Over the course of our project we want to find out which mutagenesis system is most suitable to our directed evolution approach.  
 
Over the course of our project we want to find out which mutagenesis system is most suitable to our directed evolution approach.  
 
Therefore we will compare both possibilities in terms of mutagenesis rate, -spectrum, -controllability and -specifity. How will  
 
Therefore we will compare both possibilities in terms of mutagenesis rate, -spectrum, -controllability and -specifity. How will  
we do this? Find out on our <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation">mutation page</a>.
+
we do this? Find out on our <a href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation">mutation</a> mainpage.
 
+
 
</div>
 
</div>
 +
<br>
 +
<br>
 +
<center>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Library" role="button"><button>Library</button></a>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Mutation" role="button"><button>Mutation</button></a>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Project/Selection/Motivation" role="button"><button>Selection</button></a>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Model" role="button"><button>Modeling</button></a>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Results" role="button"><button>Results</button></a>
 +
</center>
 
 
 
<br><br><br>
 
<br><br><br>
Line 492: Line 160:
 
<div class="container text_header">
 
<div class="container text_header">
 
<h2>Improve a part</h2>
 
<h2>Improve a part</h2>
<h3>Mutator gene dnaQ926 - BBa_K1333108</h3>
+
<h3>Mutator gene dnaQ926 - <a href="http://parts.igem.org/Part:BBa_K1333108">BBa_K1333108</a></h3>
<h3>Introduction</h3>
+
 
</div>
 
</div>
 
<div class="container text">
 
<div class="container text">
DnaQ is part of the DNA polymerase III and is responsible for the proofreading activity of this complex. The dnaQ926 variant
+
We used <a href="https://2014.igem.org/Team:SYSU-China">iGEM SYSU-China 2014's</a> dnaQ926 (<a href="http://parts.igem.org/Part:BBa_K1333108">BBa_K1333108</a>) in our genome wide mutator.
loses this activity through mutation of two function essential amino acids inside the active site. The complete loss of proofreading
+
<br>
as well as the resulting saturation of mismatch-repair makes dnaQ926 the single strongest mutator gene known. (Fijalkowska und Schaaper 1996)
+
See <a href="">here</a> or go directly to the <a href="http://parts.igem.org/Part:BBa_K1333108">partsreg</a> to see how we contribute to BBa_K1333108 characterization.
 
</div>
 
</div>
 +
<br>
 +
<br>
 +
<center>
 +
<a class= "button_link" href="https://2016.igem.org/Team:Bielefeld-CeBiTec/Parts/Improve" role="button"><button>Improve a part</button></a>
 +
</center>
 
<hr>
 
<hr>
 
<div class="container text_header"><h3>Literature</h3></div>
 
<div class="container text_header"><h3>Literature</h3></div>
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<li id="Badran2015">Badran, Ahmed H.; Liu, David R. (2015): Development of potent in vivo mutagenesis plasmids with broad mutational spectra. In: Nature communications 6, S. 8425. DOI: 10.1038/ncomms9425.</li>
 
<li id="Badran2015">Badran, Ahmed H.; Liu, David R. (2015): Development of potent in vivo mutagenesis plasmids with broad mutational spectra. In: Nature communications 6, S. 8425. DOI: 10.1038/ncomms9425.</li>
 
<li id="Camps2010">Camps, Manel (2010): Modulation of ColE1-like plasmid replication for recombinant gene expression. In: Recent patents on DNA & gene sequences 4 (1), S. 58–73.</li>
 
<li id="Camps2010">Camps, Manel (2010): Modulation of ColE1-like plasmid replication for recombinant gene expression. In: Recent patents on DNA & gene sequences 4 (1), S. 58–73.</li>
<li id="Camps2003">Camps, Manel; Naukkarinen, Jussi; Johnson, Ben P.; Loeb, Lawrence A. (2003): Targeted gene evolution in Escherichia coli using a highly error-prone DNA polymerase I. In: Proceedings of the National Academy of Sciences of the United States of America 100 (17), S. 9727–9732. DOI: 10.1073/pnas.1333928100.</li>
+
<li id="Camps2003">Camps, Manel; Naukkarinen, Jussi; Johnson, Ben P.; Loeb, Lawrence A. (2003): Targeted gene evolution in Escherichia&nbsp;coli using a highly error-prone DNA polymerase I. In: Proceedings of the National Academy of Sciences of the United States of America 100 (17), S. 9727–9732. DOI: 10.1073/pnas.1333928100.</li>
<li id="Fijalkowsk1996">Fijalkowska, I. J.; Schaaper, R. M. (1996): Mutants in the Exo I motif of Escherichia coli dnaQ: defective proofreading and inviability due to error catastrophe. In: Proceedings of the National Academy of Sciences of the United States of America 93 (7), S. 2856–2861.</li>
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<li id="Fijalkowsk1996">Fijalkowska, I. J.; Schaaper, R. M. (1996): Mutants in the Exo I motif of Escherichia&nbsp;coli dnaQ: defective proofreading and inviability due to error catastrophe. In: Proceedings of the National Academy of Sciences of the United States of America 93 (7), S. 2856–2861.</li>
<li id="Greener1997">Greener, A.; Callahan, M.; Jerpseth, B. (1997): An efficient random mutagenesis technique using an E. coli mutator strain. In: Molecular biotechnology 7 (2), S. 189–195. DOI: 10.1007/BF02761755.</li>
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<li id="Greener1997">Greener, A.; Callahan, M.; Jerpseth, B. (1997): An efficient random mutagenesis technique using an <i>E.&nbsp;coli</i> mutator strain. In: Molecular biotechnology 7 (2), S. 189–195. DOI: 10.1007/BF02761755.</li>
 
<li id="Teng2007">Teng, Grace; Papavasiliou, F. Nina (2007): Immunoglobulin somatic hypermutation. In: Annual review of genetics 41, S. 107–120. DOI: 10.1146/annurev.genet.41.110306.130340.</li>
 
<li id="Teng2007">Teng, Grace; Papavasiliou, F. Nina (2007): Immunoglobulin somatic hypermutation. In: Annual review of genetics 41, S. 107–120. DOI: 10.1146/annurev.genet.41.110306.130340.</li>
 
</ul>
 
</ul>
 
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Latest revision as of 14:58, 7 December 2016



Project Description

The only way to do great work is to love what you do - Steve Jobs

Motivation

As long as mankind remembers, different diseases struck from time to time and demanded millions of lives. Maybe the most fatal of these epidemic outbreaks was the 1918 flu pandemic, which killed between 50-100 million people worldwide. Derived from a simple influenza virus only a few mutations were necessary to change this virus into one of the deadliest threats that ever existed. Pandemic viral infections like this were the reason for our project selection. Our highest motivation was to create a system to counteract these extremely high risk potential slumbering in commonly known and seemingly not to dangerous viruses. Of course the influenza virus stated 1918 a much higher risk than it does today. But still viruses are very hard to treat and especially members of the family flaviviridae like Zika or Dengue virus, show a high risk potential because of their high mutation rate.
We found a way to create in a short period of time antibody-like proteins. Evobodies are binding proteins that are able to be quickly adapted to altered targets like viral hull proteins and re-establish binding properties in extremely short periods of time The limiting factors in this process are the rate at which mutations happen in the gene of the Evobody and screening of different proteins. This is the reason why we wanted to build a mutation inducing system which is not only able to change basepairs in vivo at a very high frequency, but is also specific enough to provide stability in culture and does not interfere too much with growth properties of the individual cell.
The revolutionary part of Evobody generation is the combination of an in vivo mutagenesis and a selection system which is also capable of screening our mutants during the process of cell cultivation. Due to our constant interaction of altered binding proteins and the in vivo selection, we were eager to increase the mutation rate while retaining normal growth conditions. That is why we did not only calculate the mutation rate of our two different mutagenesis approaches, but also determined the growth rate under different conditions.

Generation of binding proteins by directed evolution

This year the iGEM Team Bielefeld-CeBiTec aims to create a method for generating synthetic binding proteins, our so-called Evobodies. This works by creating a library of binding proteins and increasing their affinity towards a target by directed evolution (Figure 1). As a starting point, we randomize the binding regions of synthetic antibody-like proteins (Figure 1A). Following we screen this library for affinity towards a target by using a bacterial two-hybrid system (Figure 1B). To further increase the Evobodies affinity, we combine the selection via the two-hybrid system with an in vivo mutagenesis system (Figure 1C). Doing this we hope to generate strong and specific binding proteins by combining the powerful genetics of E. coli with the biological idea of antibody generation and maturation in vertebrates.
Figure 1: Schematic Evobody generation process. A library of synthetic binding proteins (A) is screened by a bacterial two hybrid(B) for interaction with a traget protein. Existing interaction between both proteins leads to expression of a resistance gene thus granting the individual cell a selection advantage. After screening the library all suviving clones binding proteins are mutagenized in vivo (C) which results in the generation of new binding properties. Continuous selection cycles of selection and mutation increase the Evobodies binding affinity towards high affine binding proteins.
We designed our Evobody approach as an alternative to conventional methods for the generation of binding proteins. In our vision it should be possible to clone each protein encoding sequence into one of our plasmids, let our system do the work and get a high affinity binding protein, which can be either used for medical, diagnostic or scientific applications.

The starting point - synthetic binding protein library

As starting point, we want to create a library of many binding proteins with a high chance to contain a protein with the potential to bind our target protein. In doing so we choose the core region of the antibody-mimetic mono- and nanobodies. In the coding region of those proteins, we randomized the loop regions, which are known to bind other proteins to obtain our library.
The randomization strategy as well as the choice of the protein scaffold is a key part of library generation. We identified amino acids, which are present in most protein-protein interaction areas and created a randomization scheme so that only these amino acids are encoded in the antibody-mimetics binding region. Read more about our library design here.



Figure 2: Library of initial binding proteins. Expression of the initial binding proteins with variable regions highlighted in seperate colors (turquoise, orange, white, green, pink and blue) and constant regions in olive. The theoretical variability for each scaffold is 1.073.741.824.

Survival of the fittest - bacterial two-hybrid

In the next step, the binding protein library should be screened for proteins with an innate affinity for our target. We want to realize this by using a bacterial two-hybrid system (Figure 3). Therefore, our target protein (1) is fused to a DNA binding domain (2), which localises upstream of a reporter cassette (3). The binding protein (4) is fused to a RNA polymerase subunit (5). Interaction between the binding and the target protein leads to recruitment of the RNA polymerase to the promoter region of the reporter cassette and activates the reporter gene expression. By using an antibiotic resistance as a reporter gene the output of the bacterial two hybrid system should lead to the survival E. coli cells carrying a good binding protein and the death of all cells with a bad binding protein.
Figure 3: Bacterial-two hybrid system.Interaction between the binding protein (4) and the target protein (1) lead to recruitment of RNA polymerase (5) to the promoter upstream of the reporter cassette (3) and subsequent expression of the reporter gene. In this case the reporter is beta-lactamase, which expression leads to degradation of ampicillin (blue squares) and survival of the bacteria.
From the two-hybrid system we expect foremost a selection of the binding protein library. Furthermore, we expect a correlation between binding - target protein affinity and the activated gene expression strength of the reporter. By using an antibiotic resistance protein as a reporter we predict increased levels of the resistance protein inside a cell with a high affinity binding protein. The outcome of this should be an increase of individual fitness for bacteria with good binding proteins, which should lead to a higher growth rate under strong selective pressure. The complete two-hybrid system should cumulate in a correlation between binding protein affinity and bacterial growth rate, which should lead to selection of a few bacteria with strong binding proteins. Find out more on our selection subpage.

Accessing the sequence space - in vivo mutagenesis

After selection of the bulk of our library we will increase the affinity of our Evobodies in a process similar to the affinity maturation of antibodies (Teng und Papavasiliou 2007). As addressed above we will select our Evobodies by increasing the selection pressure. At the same time, we will use an in vivo mutagenesis system. Thereby ,we can increase the sequence diversity beyond the limits of our library. Slightly modifications of binding proteins identified during the initial selection will are the basis for the directed evolution.
Figure 4: In vivo mutagenesis system. By using an in vivo mutagenesis system a single Evobody coding sequence can be evolved to various different variants, each with a unique binding site. The single starting sequence is replicated during growth and thereby mutations are incorporated either through error-prone polymerase I or a combination of global mutator genes. The process results in the creating of the library of binding proteins with different binding properties.

In detail, we will compare two different possibilities to diversify our binding proteins. The first approach is the use of an error-prone polymerase I in an otherwise Pol I temperature-sensitive E. coli strain. (Camps et al. 2003) Growth at a non-permissive temperature should result in accumulation of mutations in the part of the genom maintained by DNA polymerase I. The interesting idea behind this approach is the fact that large parts of plasmids carrying an origin of replication from the ColE1-familiy are replicated by the polymerase I. (Camps et al. 2003; Camps 2010) Because of this, the usage of the error-prone polymerase I should mutant mainly our Evobody sequence on a plasmid. Thereby off-target mutations, which are a major obstacle of in vivo mutagenesis, should be minimized. (Camps et al. 2003)
Our other approach is based on creating a plasmid borne hypermutator system by modulating the E. coli DNA fidelity systems. (Badran und Liu 2015) We will express known mutator genes under tight regulation from a plasmid. By using a plasmid borne mutator system, in contrast to the more classical approaches of incorporating the mutator genes directly inside the genom. (Agilent Technologies; Greener et al. 1997) Thereby we want to circumvent the known problems with globally increased mutation rate, which are genetic instability or general unviability.
Over the course of our project we want to find out which mutagenesis system is most suitable to our directed evolution approach. Therefore we will compare both possibilities in terms of mutagenesis rate, -spectrum, -controllability and -specifity. How will we do this? Find out on our mutation mainpage.





Improve a part

Mutator gene dnaQ926 - BBa_K1333108

We used iGEM SYSU-China 2014's dnaQ926 (BBa_K1333108) in our genome wide mutator.
See here or go directly to the partsreg to see how we contribute to BBa_K1333108 characterization.



Literature

  • Agilent Technologies: XL1-Red Competent Cells. Instruction Manual 2015.
  • Badran, Ahmed H.; Liu, David R. (2015): Development of potent in vivo mutagenesis plasmids with broad mutational spectra. In: Nature communications 6, S. 8425. DOI: 10.1038/ncomms9425.
  • Camps, Manel (2010): Modulation of ColE1-like plasmid replication for recombinant gene expression. In: Recent patents on DNA & gene sequences 4 (1), S. 58–73.
  • Camps, Manel; Naukkarinen, Jussi; Johnson, Ben P.; Loeb, Lawrence A. (2003): Targeted gene evolution in Escherichia coli using a highly error-prone DNA polymerase I. In: Proceedings of the National Academy of Sciences of the United States of America 100 (17), S. 9727–9732. DOI: 10.1073/pnas.1333928100.
  • Fijalkowska, I. J.; Schaaper, R. M. (1996): Mutants in the Exo I motif of Escherichia coli dnaQ: defective proofreading and inviability due to error catastrophe. In: Proceedings of the National Academy of Sciences of the United States of America 93 (7), S. 2856–2861.
  • Greener, A.; Callahan, M.; Jerpseth, B. (1997): An efficient random mutagenesis technique using an E. coli mutator strain. In: Molecular biotechnology 7 (2), S. 189–195. DOI: 10.1007/BF02761755.
  • Teng, Grace; Papavasiliou, F. Nina (2007): Immunoglobulin somatic hypermutation. In: Annual review of genetics 41, S. 107–120. DOI: 10.1146/annurev.genet.41.110306.130340.