Team:Tokyo Tech/Projects/RPS-game/index.htm

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<li><a href="https://2011.igem.org/Team:Tokyo_Tech/notebook">NoteBook</a></li>
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/notebook">NoteBook</a></li>
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/team">Team</a></li>
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/team">Team</a></li>
-
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/Sponsers.htm">Sponsers</a></li>
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<li><a href="https://2011.igem.org/Team:Tokyo_Tech/Sponsers.htm">Sponsors</a></li>
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/Collaboration.htm">Collaboration</a></li>
<li><a href="https://2011.igem.org/Team:Tokyo_Tech/Collaboration.htm">Collaboration</a></li>
</ul>
</ul>
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<div style="min-height: 20600px; float: left;">
<div id="LeftMenu">
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<li><a href="#1">1. The Hands</a></li>
<li><a href="#1">1. The Hands</a></li>
<li>
<li>
-
<a href="#2">2. The Judge</a>
+
<a href="#2">2. The Judges</a>
<ul>
<ul>
<li><a href="#2.1">2.1 Using AND-Gate promoters to create Judges</a></li>
<li><a href="#2.1">2.1 Using AND-Gate promoters to create Judges</a></li>
<li><a href="#2.2">2.2 Creating Parts that responded correctly to our set of Signaling Molecules</a></li>
<li><a href="#2.2">2.2 Creating Parts that responded correctly to our set of Signaling Molecules</a></li>
<li><a href="#2.3">2.3 Improving PlsrA</a></li>
<li><a href="#2.3">2.3 Improving PlsrA</a></li>
-
<li><a href="#2.4">2.4 Improving PlasI</a></li>
+
<li><a href="#2.4">2.4 Improving Plas</a></li>
</ul>
</ul>
</li>
</li>
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<li><a href="#3.2.1">3.2.1 The Requirements</a></li>
<li><a href="#3.2.1">3.2.1 The Requirements</a></li>
<li><a href="#3.2.2">3.2.2 The Mechanism</a></li>
<li><a href="#3.2.2">3.2.2 The Mechanism</a></li>
-
<li><a href="#3.2.3">3.2.3 Testing the Lox Cassettes</a></li>
+
<li><a href="#3.2.3">3.2.3 Testing the <i>Lox</i> Cassettes</a></li>
<li><a href="#3.2.4">3.2.4 Playing Fair: Future Work</a></li>
<li><a href="#3.2.4">3.2.4 Playing Fair: Future Work</a></li>
</ul>
</ul>
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<a href="#3.3">3.3 Survival of one strain</a>
<a href="#3.3">3.3 Survival of one strain</a>
<ul>
<ul>
-
<li><a href="#3.3.1">3.3.1 Introduction: Minimal differences determine who will survive</a></li>
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<li><a href="#3.3.1">3.3.1 Introduction: Very small differences determine who will survive</a></li>
<li><a href="#3.3.2">3.3.2 Adjusting the Model to create a True Randomizer</a></li>
<li><a href="#3.3.2">3.3.2 Adjusting the Model to create a True Randomizer</a></li>
<li><a href="#3.3.3">3.3.3 How the Three Types of Bacteria Compete for Survival</a></li>
<li><a href="#3.3.3">3.3.3 How the Three Types of Bacteria Compete for Survival</a></li>
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<div align= "center">
<div align= "center">
<span class="top"> The Hands </span><br />
<span class="top"> The Hands </span><br />
-
<img src="https://static.igem.org/mediawiki/2011/1/13/Handzu.png" width="300px" />
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<img src="https://static.igem.org/mediawiki/2011/4/48/Jyangken.png" width="300px" />
</div>
</div>
<p>
<p>
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two sets of three signaling molecules corresponding each to rock, paper or scissors.  
two sets of three signaling molecules corresponding each to rock, paper or scissors.  
For humans we used IPTG, aTc and salicylate, respectively.  
For humans we used IPTG, aTc and salicylate, respectively.  
-
For E. coli we used 3OC6-HSL, 3OC12-HSL and AI-2, respectively.
+
For <span class="name">E. coli</span> we used 3OC6-HSL, 3OC12-HSL and AI-2, respectively.
</p>
</p>
<hr />
<hr />
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<tr>
<tr>
<td><img src="https://static.igem.org/mediawiki/2011/2/24/BBa_K649001_graph3.png" width="360px" /></td>
<td><img src="https://static.igem.org/mediawiki/2011/2/24/BBa_K649001_graph3.png" width="360px" /></td>
-
<td><img src="http://partsregistry.org/wiki/images/f/f4/LsrA_promoter_activity_introduction.png" width="400px" /></td>
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<td><img src="https://static.igem.org/mediawiki/2011/f/fb/PlsrA3.png" width="400px" /></td>
</tr>
</tr>
</table>
</table>
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Although our set of six signaling molecules allows us to play RPS with  
Although our set of six signaling molecules allows us to play RPS with  
<span class="name">E. coli</span>, we must make sure <span class="name">E. coli</span>  
<span class="name">E. coli</span>, we must make sure <span class="name">E. coli</span>  
-
can chose any of its three signaling molecules with the same probability  
+
can choose any of its three signaling molecules with the same probability  
in order to be able to play RPS fairly and properly.  
in order to be able to play RPS fairly and properly.  
To do so, we designed three kinds of randomizers.
To do so, we designed three kinds of randomizers.
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<p>
<p>
<h2 id="1">1. The Hands</h2>
<h2 id="1">1. The Hands</h2>
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<img src="https://static.igem.org/mediawiki/2011/4/4b/Image001.png" width="600px" style="float:right;"/>
+
<img src="https://static.igem.org/mediawiki/2011/7/75/The_hands.png" width="600px" style="float:right;" />
<p>
<p>
The first step towards making an RPS game that can be played between  
The first step towards making an RPS game that can be played between  
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</p>
</p>
                  
                  
-
<h2 id="2" style="clear:both;">2. The Judge</h2>
+
<h2 id="2" style="clear:both;">2. The Judges</h2>
-
        <img src="https://static.igem.org/mediawiki/2011/8/8a/Judge.png" alt="the Judge" style="float: left;" />
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<img src="https://static.igem.org/mediawiki/2011/8/8a/Judge.png" alt="the Judge" style="float: left;" />
<p>
<p>
Although we defined a set of six signaling molecules that can be used  
Although we defined a set of six signaling molecules that can be used  
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Our next mission was then to check if there were AND-gate promoters BioBricks  
Our next mission was then to check if there were AND-gate promoters BioBricks  
that we could use. We searched in the Registry and found a potential AND-gate  
that we could use. We searched in the Registry and found a potential AND-gate  
-
promoter designed by iGEM 2007's team Tokyo Alliance. This potential AND-gate  
+
promoter designed by iGEM 2007's team Tokyo_Tech. This potential AND-gate  
-
promoter is designed to be activated by the addition of both IPTG and 3O-C6-HSL.  
+
promoter is designed to be activated by the addition of both IPTG and 3OC6-HSL.  
However, there was no data showing the IPTG dependency of this promoter,  
However, there was no data showing the IPTG dependency of this promoter,  
so we did experiments and confirmed this dependency for the first time in iGEM.  
so we did experiments and confirmed this dependency for the first time in iGEM.  
-
We concluded that the addition of both IPTG and 3O-C6-HSL regulates the activity  
+
We concluded that the addition of both IPTG and 3OC6-HSL regulates the activity  
of this AND-gate promoter. In this way, we completed the construction of one of  
of this AND-gate promoter. In this way, we completed the construction of one of  
the Judges <span class="name">E. coli</span>, which proves in principle that  
the Judges <span class="name">E. coli</span>, which proves in principle that  
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<div style="float:left">
<div style="float:left">
-
<img src="https://static.igem.org/mediawiki/2011/b/be/BBa_I751101_graph3.png" width="400px" /><br />
+
<img src="https://static.igem.org/mediawiki/2011/b/be/BBa_I751101_graph3.png" width="400px" style="margin-right: 10px;"/><br />
-
<span class="graph_title">Fig 2.1 Tokyo Alliance AND-gate promoter</span>
+
<span class="graph_title">Fig. 2.1 Tokyo_Tech AND-gate promoter</span>
</div>
</div>
<p>
<p>
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controls the binding of LuxR to a LuxR-operator part, the <span class="gene">gfp</span>  
controls the binding of LuxR to a LuxR-operator part, the <span class="gene">gfp</span>  
gene activity of the reporter part is dually regulated by IPTG and 3OC6-HSL.  
gene activity of the reporter part is dually regulated by IPTG and 3OC6-HSL.  
-
We used promoterless pSB3K3-gfp (BBa_J54103) as a negative control,  
+
We used promoterless pSB3K3-<span class="gene">gfp</span> (BBa_J54103) as a negative control,  
-
and pAC-P&lambda;-gfp (chloramphenicol-resistance), which constitutively expressed GFP,  
+
and pAC-P&lambda;-<span class="gene">gfp</span> (chloramphenicol-resistance), which constitutively expressed GFP,  
as a positive control. To know about the mechanism of this promoter click  
as a positive control. To know about the mechanism of this promoter click  
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#4.0.">here</a>.
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#4.0.">here</a>.
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<p>
<p>
In the process of constructing enough AND-gates that could suffice the needs  
In the process of constructing enough AND-gates that could suffice the needs  
-
of our RPS game design, we discovered two faulty BioBricks: PlsrA (BBa_K117002) and PlasI (BBa_J64010).  
+
of our RPS game design, we discovered two faulty BioBricks: lsrA promoter (BBa_K117002) and las promoter (BBa_J64010).  
Because of these faulty parts, the Judge <span class="name">E. coli</span>  
Because of these faulty parts, the Judge <span class="name">E. coli</span>  
set we had designed could only sense the Player <span class="name">E. coli</span>'s  
set we had designed could only sense the Player <span class="name">E. coli</span>'s  
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</p>
</p>
<p>
<p>
-
To fix this problem, we improved the old defective lasI and lsrA promoters parts  
+
To fix this problem, we improved the old defective las and lsrA promoters parts  
by making new parts that work! As can be seen in the experimental information  
by making new parts that work! As can be seen in the experimental information  
-
below (see “Improving PlsrA” and “Improving PlasI”),  
+
below (see “Improving lsrA promoter” and “Improving las promoter”),  
-
we confirmed our PlasI (<a href="http://partsregistry.org/Part:BBa_K649000">BBa_K649000</a>)  
+
we confirmed our lasI promoter (<a href="http://partsregistry.org/Part:BBa_K649000">BBa_K649000</a>)  
-
and PlsrA (<a href="http://partsregistry.org/Part:BBa_K649100">BBa_K649100</a>) work perfectly!
+
and lsrA promoter (<a href="http://partsregistry.org/Part:BBa_K649100">BBa_K649100</a>) work perfectly!
</p>
</p>
<p>
<p>
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reference to construct AND gate promoters. Therefore, we solved important issues  
reference to construct AND gate promoters. Therefore, we solved important issues  
and made significant advances towards constructing AND-gate promoters. This allows  
and made significant advances towards constructing AND-gate promoters. This allows  
-
<span class="name">E. coli</span> to also chose the signaling molecules  
+
<span class="name">E. coli</span> to also choose the signaling molecules  
corresponding to Paper and Scissors, so we have again a working RPS game design.
corresponding to Paper and Scissors, so we have again a working RPS game design.
</p>
</p>
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<div style="float: left;">
<div style="float: left;">
-
<img src="http://partsregistry.org/wiki/images/3/33/LsrA_promoter_activity.png" alt="activity" width="400px" /><br />
+
<img src="https://static.igem.org/mediawiki/2011/6/6e/PlsrA2.png" alt="activity" width="400px" /><br />
-
<span class="graph_title">Fig 2.2 Not working lsrA promoter(BBa_K117002) <br /> activity and our new lsrA promoter(BBa_K649100)</span> activity
+
<span class="graph_title">Fig. 2.2 Not working lsrA promoter(<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>) <br /> activity and our new lsrA promoter(<a href="http://partsregistry.org/Part:BBa_K649104">BBa_K649104</a>)</span> activity
</div>
</div>
<p>
<p>
-
We confirmed that the lsrA promoter (BBa_K117002) does not work properly  
+
We confirmed that the lsrA promoter (<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>) does not work properly  
-
(samples used our experiment are listed in Table 2.1 below). The fluorescence intensity of GFP of lsrA promoter-gfp((BBa_K117002)-gfp) was lower  
+
(samples used our experiment are listed in Table 2.1 below). The fluorescence intensity of GFP of lsrA promoter-<span class="gene">gfp</span>((<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>)-<span class="gene">gfp</span>) was lower  
-
even than those of the negative control (Fig.2.2), which clearly shows that  
+
even than those of the negative control (Fig. 2.2), which clearly shows that  
-
lsrA promoter(BBa_K117002) does not work as expected. In this experiment,  
+
lsrA promoter((<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>) does not work as expected. In this experiment,  
we measured transcriptional activity of lsrA promoter by introducing a  
we measured transcriptional activity of lsrA promoter by introducing a  
-
<span class="gene">gfp</span> gene downstream of this promoter (Fig.2.3).
+
<span class="gene">gfp</span> gene downstream of this promoter (Fig. 2.3).
</p>
</p>
-
+
 
-
<table style="clear:both;" border="1" align="center">
+
<table style="clear:both;margin-top: 20px;" border="1" align="center">
<caption>Table 2.1 Samples used our experiment</caption>
<caption>Table 2.1 Samples used our experiment</caption>
<tr>
<tr>
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<td>sample1</td>
<td>sample1</td>
<td rowspan="4">JD22597</td>
<td rowspan="4">JD22597</td>
-
<td>Ptet-gfp on pSB1A2</td>
+
<td>Ptet-<span class="gene">gfp</span> on pSB1A2</td>
</tr>
</tr>
<tr>
<tr>
<td>sample2</td>
<td>sample2</td>
-
<td>Promoterless-gfp on pSB6A1</td>
+
<td>Promoterless-<span class="gene">gfp</span> on pSB6A1</td>
</tr>
</tr>
<tr>
<tr>
<td>sample3</td>
<td>sample3</td>
-
<td>PlsrA-gfp on pSB1A2 (<a href="http://partsregistry.org/Part:BBa_K649104">BBa_K649104</a>)</td>
+
<td>PlsrA-<span class="gene">gfp</span> on pSB1A2 (<a href="http://partsregistry.org/Part:BBa_K649104">BBa_K649104</a>)</td>
</tr>
</tr>
<tr>
<tr>
<td>sample4</td>
<td>sample4</td>
-
<td>PlsrA-gfp on pSB1A2 ((<a href="http://partsregistry.org/Part:>BBa_K117002">BBa_K117002</a>)-gfp)</td>
+
<td>PlsrA-<span class="gene">gfp</span> on pSB1A2 ((<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>)-<span class="gene">gfp</span>)</td>
</tr>
</tr>
</table>
</table>
          
          
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/9/92/Lasr3.png" alt="Fig2.3" width="200px" /><br />
+
<img src="https://static.igem.org/mediawiki/2011/f/fb/PlsrAo.png" alt="Fig2.3" width="200px" /><br />
-
<span class="graph_title">Fig2.3 lsrA promoter-gfp((BBa_K117002)-gfp)</span>
+
<span class="graph_title">Fig. 2.3 lsrA promoter-<span class="gene">gfp</span>((<a href="http://partsregistry.org/Part:BBa_K117002">BBa_K117002</a>)-<span class="gene">gfp</span>)</span>
</div>
</div>
<p>
<p>
-
To solve this problem, we created the first working iGEM lsrA promoter (BBa_K649100).  
+
To solve this problem, we created the first working iGEM lsrA promoter (<a href="http://partsregistry.org/Part:BBa_K649100">BBa_K649100</a>).  
Its fluorescence intensity was much higher than that from a promoter-less  
Its fluorescence intensity was much higher than that from a promoter-less  
<span class="gene">gfp</span> negative control plasmid, showing that our new  
<span class="gene">gfp</span> negative control plasmid, showing that our new  
-
lsrA promoter works(Fig2.5). In this experiment, we measured the transcriptional  
+
lsrA promoter works(Fig. 2.5). In this experiment, we measured the transcriptional  
-
activity of our lsrA promoter by introducing a gfp gene downstream of  
+
activity of our lsrA promoter by introducing a <span class="gene">gfp</span> gene downstream of  
-
the promoter(BBa_K649104, Fig2.4). Details about this experiment can be found  
+
the promoter(<a href="http://partsregistry.org/Part:BBa_K649104">BBa_K649104</a>, Fig. 2.4). Details about this experiment can be found  
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#5.">here</a>.
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#5.">here</a>.
</p>
</p>
   
   
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/f/ff/Lasr4.png" alt="Fig2.4" width="200px"><br />
+
<img src="https://static.igem.org/mediawiki/2011/6/60/PlsrAgfpx.png" alt="Fig2.4" width="200px"><br />
-
<span class="graph_title">Fig 2.4 lsrA promoter-gfp(BBa_K649104)</span>
+
<span class="graph_title">Fig. 2.4 lsrA promoter-<span class="gene">gfp</span>(<a href="http://partsregistry.org/Part:BBa_K649104">BBa_K649104</a>)</span>
-
</div>
+
</div> <br />
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/6/6d/LsrR_repression1.png" alt="Fig4" width="600px"><br />
+
<img src="https://static.igem.org/mediawiki/2011/archive/6/6d/20111028133941%21LsrR_repression1.png" alt="Fig4" width="600px"><br />
-
<span class="graph_title">Fig2.5. LsrR represses lsrA promoter.</span>
+
<span class="graph_title">Fig. 2.5 LsrR represses lsrA promoter.</span>
</div>
</div>
<p>
<p>
-
Moreover, this promoter can be repressed by our new LsrR part(BBa_K649105).  
+
Moreover, this promoter can be repressed by our new LsrR part(<a href="http://partsregistry.org/Part:BBa_K649105">BBa_K649105</a>).  
(samples used our experiments are listed in Table 2.2 below) The fluorescence  
(samples used our experiments are listed in Table 2.2 below) The fluorescence  
intensity of GFP of sample 3 was three times as large as  
intensity of GFP of sample 3 was three times as large as  
that of sample 4. This result shows that LsrR successfully repressed  
that of sample 4. This result shows that LsrR successfully repressed  
lsrA promoter. In this experiment, we measured LsrR repression activity by  
lsrA promoter. In this experiment, we measured LsrR repression activity by  
-
introducing a gfp gene downstream of lsrA promoter (BBa_K649105, Fig.2.6).
+
introducing a <span class="gene">gfp</span> gene downstream of lsrA promoter ((<a href="http://partsregistry.org/Part:BBa_K649105">BBa_K649105</a>, Fig. 2.6).
Details about this experiment can be found  
Details about this experiment can be found  
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#6.">here</a>.
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#6.">here</a>.
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<td>sample1</td>
<td>sample1</td>
<td rowspan="2">JM2.300</td>
<td rowspan="2">JM2.300</td>
-
<td>Ptet-gfp on pSB6A1</td>
+
<td>Ptet-<span class="gene">gfp</span> on pSB6A1</td>
</tr>
</tr>
<tr>
<tr>
<td>sample2</td>
<td>sample2</td>
-
<td>Promoterless-gfp on pSB3K3</td>
+
<td>Promoterless-<span class="gene">gfp</span> on pSB3K3</td>
</tr>
</tr>
<tr>
<tr>
<td>sample3</td>
<td>sample3</td>
<td rowspan="2">MG1655</td>
<td rowspan="2">MG1655</td>
-
<td>PlsrA-gfp on pSB3K3</td>
+
<td>PlsrA-<span class="gene">gfp</span> on pSB3K3</td>
</tr>
</tr>
<tr>
<tr>
<td>sample4</td>
<td>sample4</td>
-
<td>PlsrA-gfp-PlsrR-lsrR on pSB3K3</td>
+
<td>PlsrA-<span class="gene">gfp</span>-PlsrR-<span class="gene">lsrR</span> on pSB3K3</td>
</tr>
</tr>
</table>
</table>
   
   
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/b/b2/Lasr7.png" alt="Fig.5" width="200px"><br />
+
<img src="https://static.igem.org/mediawiki/2011/d/dc/PlsrAPlsrR.png" alt="Fig.5" width="200px"><br />
-
<span class="graph_title">Fig2.6 lsrA promoter-gfp-lsrR promoter-lsrR(BBa_K649105)</span>
+
<span class="graph_title">Fig. 2.6 lsrA promoter-<span class="gene">gfp</span>-lsrR promoter-<span class="gene">lsrR</span>(<a href="http://partsregistry.org/Part:BBa_K649105">BBa_K649105</a>)</span>
</div>
</div>
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<td>
<td>
                         <img src="https://static.igem.org/mediawiki/2011/8/80/BBa_J64010_graph3.png" align="left" height="330px" />
                         <img src="https://static.igem.org/mediawiki/2011/8/80/BBa_J64010_graph3.png" align="left" height="330px" />
-
                         <span class="graph_title">Fig2.7 (a)</span>
+
                         <span class="graph_title">Fig. 2.7 (a)</span>
                         </td>
                         </td>
<td>
<td>
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</table>
</table>
<p>
<p>
-
Fig2.7 (a): Not working lasI promoter (BBa_J64010).  
+
Fig. 2.7 (a): Not working lasI promoter (BBa_J64010).  
-
Fig2.7 (b): New working lasI promoter (BBa_K649000) we made.  
+
Fig. 2.7 (b): New working lasI promoter (BBa_K649000) we made.  
We confirmed it works as expected. In our assay, we used the same LasR  
We confirmed it works as expected. In our assay, we used the same LasR  
regulator part used in the assay of BBa_ J64010. Clearly, for our  
regulator part used in the assay of BBa_ J64010. Clearly, for our  
Line 676: Line 676:
Although our set of six signaling molecules allows us to play RPS with  
Although our set of six signaling molecules allows us to play RPS with  
<span class="name">E. coli</span>, we must make sure <span class="name">E. coli</span>  
<span class="name">E. coli</span>, we must make sure <span class="name">E. coli</span>  
-
can chose any of its three signaling molecules with the same probability  
+
can choose any of its three signaling molecules with the same probability  
in order to be able to play RPS fairly and properly. To do so, we designed  
in order to be able to play RPS fairly and properly. To do so, we designed  
three kinds of randomizers: one kind which needs of three types of bacteria  
three kinds of randomizers: one kind which needs of three types of bacteria  
Line 691: Line 691:
<p>
<p>
This is our simplest randomizer design. To make sure <span class="name">E. coli</span>  
This is our simplest randomizer design. To make sure <span class="name">E. coli</span>  
-
choses any of its signaling molecules with equal probability, we put the constructs  
+
chooses any of its signaling molecules with equal probability, we put the constructs  
for each molecule inside a different bacterium, so we create three types of bacteria:  
for each molecule inside a different bacterium, so we create three types of bacteria:  
one synthetizing the corresponding signaling molecule for rock, other synthetizing  
one synthetizing the corresponding signaling molecule for rock, other synthetizing  
Line 704: Line 704:
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/6/69/742px-Image136.png" width="550px" align="center" />
+
<img src="https://static.igem.org/mediawiki/2011/0/0c/Cre-lox_mechanism_1.png" width="550px" align="center" />
</div>
</div>
<p>
<p>
Line 714: Line 714:
We designed a Cre-Lox system which allows <span class="name">E. coli</span>  
We designed a Cre-Lox system which allows <span class="name">E. coli</span>  
to express one of its three signaling molecules by means of conditional knockout.  
to express one of its three signaling molecules by means of conditional knockout.  
-
The design is depicted in Fig 1. It should be noted this randomizer is designed  
+
The design is depicted in Fig. 1. It should be noted this randomizer is designed  
to be used at a single-cell level. When this randomizer is used in groups of cells,  
to be used at a single-cell level. When this randomizer is used in groups of cells,  
the different signals released by the cells will mix. In this case, by using microfluidic  
the different signals released by the cells will mix. In this case, by using microfluidic  
Line 722: Line 722:
<div align="center">
<div align="center">
-
<span class="graph_title">(a)</span>
+
<img src="https://static.igem.org/mediawiki/2011/3/3d/Fig_3.1_-_in_one_cell_1.png" width="700px" align="center" />
-
<img src="https://static.igem.org/mediawiki/2011/d/d4/%28a%29pbad.araC-cre.png" />
+
</div>
</div>
-
<div align="center">
+
<div class="graph_title">
-
<span class="graph_title">(b)</span>
+
Fig. 3.1 - (a) Cre recombinase construction. (b) lox cassettes distribution for the randomizer design
-
<img src="https://static.igem.org/mediawiki/2011/thumb/2/21/Image140.png/800px-Image140.png" width="700px" />
+
-
</div>
+
-
<div class="graph_title">
+
-
Fig 3.1 - (a) Cre recombinase construction. (b) Lox cassettes distribution for the randomizer design
+
</div>
</div>
Line 736: Line 731:
<p>
<p>
-
Basically, each pair of lox sites (indicated by the same color) mark the points  
+
Basically, each pair of <i>lox</i> sites (indicated by the same color) mark the points  
which the enzyme Cre will excise (they will be cut off the backbone along with the  
which the enzyme Cre will excise (they will be cut off the backbone along with the  
sequence between them). For a design that allows choosing randomly one of  
sequence between them). For a design that allows choosing randomly one of  
<span class="name">E. coli</span>’s three signaling molecules, at least two  
<span class="name">E. coli</span>’s three signaling molecules, at least two  
cassettes of lox sites are needed. When these two cassettes of lox sites and  
cassettes of lox sites are needed. When these two cassettes of lox sites and  
-
protein coding sequences are arranged as in Fig3.1(b),  
+
protein coding sequences are arranged as in Fig. 3.1(b),  
only one signaling molecule is produced.
only one signaling molecule is produced.
</p>
</p>
<p>
<p>
-
Our design also required a way to control LuxI gene's expression.  
+
Our design also required a way to control <span class="gene">luxI</span> gene's expression.  
To do so, we used an inducible promoter instead of a constitutive promoter.  
To do so, we used an inducible promoter instead of a constitutive promoter.  
-
A constitutive promoter would have caused LuxI gene to be expressed beforehand and  
+
A constitutive promoter would have caused <span class="gene">luxI</span> gene to be expressed beforehand and  
could lead to an <span class="name">E. coli</span> producing two signaling molecules  
could lead to an <span class="name">E. coli</span> producing two signaling molecules  
at the same time (the equivalent of showing two hands in the RPS game). In contrast,  
at the same time (the equivalent of showing two hands in the RPS game). In contrast,  
Line 762: Line 757:
<p>
<p>
-
When the blue cassette of Lox sites is excised (Fig 3.1), the signaling molecule  
+
When the blue cassette of <i>Lox</i> sites is excised (Fig. 3.1), the signaling molecule  
-
coded by LasI (3OC6-HSL) will be produced. Likewise, when the black Lox cassette  
+
coded by lasI (3OC6-HSL) will be produced. Likewise, when the black <i>Lox</i> cassette  
-
is excised, the signaling molecule coded by LuxS (AI-2) will be produced. On the other hand,  
+
is excised, the signaling molecule coded by luxS (AI-2) will be produced. On the other hand,  
a third possible outcome is that recombination does not take place. In this case,  
a third possible outcome is that recombination does not take place. In this case,  
-
the signaling molecule coded by LuxI (3OC6-HSL) will be produced. Also note that excision  
+
the signaling molecule coded by <span class="gene">luxI</span> (3OC6-HSL) will be produced. Also note that excision  
of one kind of lox cassette removes the remaining cassette,  
of one kind of lox cassette removes the remaining cassette,  
thereby preventing further recombination.
thereby preventing further recombination.
Line 772: Line 767:
<p>
<p>
As mentioned before, one of the requirements for our randomizer was to have at least  
As mentioned before, one of the requirements for our randomizer was to have at least  
-
two lox cassettes. This prevents excision of lox sites from different cassettes  
+
two lox cassettes. This prevents excision of <i>lox</i> sites from different cassettes  
-
(for example one blue lox site and one black lox site). Because the lox71-lox66 cassette and the lox2272-lox2272 cassette are incompatible (Zorana Carter and Daniela Delneri <i>et al.</i>, Yeast 2010), we can use them to build our randomizer.
+
(for example one blue <i>lox</i> site and one black <i>lox</i> site). Because the <i>lox71-lox66</i> cassette and the l<i>ox2272-lox2272</i> cassette are incompatible (Zorana Carter and Daniela Delneri <i>et al.</i>, Yeast 2010), we can use them to build our randomizer.
</p>
</p>
Line 780: Line 775:
<p>
<p>
As stated above, we need two lox cassettes of different recombination frequency  
As stated above, we need two lox cassettes of different recombination frequency  
-
for randomizer. Because there was no working lox parts in registry, we constructed  
+
for randomizer. Because there was no working <i>lox</i> parts in registry, we constructed  
-
three original BioBricks for testing whether lox2272 and lox7166 cassettes work. For  
+
three original BioBricks for testing whether <i>lox2272</i> and <i>lox71/66</i> cassettes work. For  
-
the convenience of testing, florescence expressing genes were used in place of signal  
+
the convenience of testing, fluorescence expressing genes were used in place of signal  
-
molecular expressing genes in construction. After figuring out their working <i>in vitro</i>, we tested them <i>in vivo</i> by detecting red and green fluorescence through fluoro imager and flow cytometer. Furthermore, we compared the relative recombination frequency of two cassettes . Our lox Cassettes constructions  
+
molecular expressing genes in construction. After figuring out their working <i>in vitro</i>, we tested them <i>in vivo</i> by detecting red and green fluorescence through fluoro imager and flow cytometer. Furthermore, we compared the relative recombination frequency of two cassettes . Our <i>lox</i> Cassettes constructions  
were working properly, and their recombination frequency were different from each other.
were working properly, and their recombination frequency were different from each other.
</p>
</p>
Line 789: Line 784:
<ul>
<ul>
<li>
<li>
-
PlacIQ-lox2272-gfp-lox2272<a href="http://partsregistry.org/Part:BBa_K649200">(BBa_649200)</a>
+
PlacIQ-<i>lox2272</i>-<span class="gene">gfp</span>-<i>lox2272</i><a href="http://partsregistry.org/Part:BBa_K649200">(BBa_K649200)</a>
-
<img src="https://static.igem.org/mediawiki/2011/d/da/Lox-gfp-lox.png" />
+
<img src="https://static.igem.org/mediawiki/2011/6/6d/Lox-gfp-lox_1.png" width="550px"/>
</li>
</li>
<li>
<li>
-
PlacIQ-lox2272-rfp-lox2272-gfp<a href="http://partsregistry.org/Part:BBa_K649201">(BBa_649201)</a>
+
PlacIQ-<i>lox2272</i>-<span class="gene">rfp</span>-<i>lox2272</i>-<span class="gene">gfp</span><a href="http://partsregistry.org/Part:BBa_K649201">(BBa_K649201)</a>
-
<img src="https://static.igem.org/mediawiki/2011/3/32/Lox-rfp-lox-gfp_2272.png" />
+
<img src="https://static.igem.org/mediawiki/2011/2/2b/Lox2272-rfp-lox-gfp_1.png" width="550px"/>
</li>
</li>
<li>
<li>
-
PlacIQ-lox71-rfp-lox66-gfp<a href="http://partsregistry.org/Part:BBa_K649202">(BBa_649202)</a>
+
PlacIQ-<i>lox71</i>-<span class="gene">rfp</span>-<i>lox66</i>-<span class="gene">gfp</span><a href="http://partsregistry.org/Part:BBa_K649202">(BBa_K649202)</a>
-
<img src="https://static.igem.org/mediawiki/2011/0/0e/Lox-rfp-lox-gfp_7166.png" />
+
<img src="https://static.igem.org/mediawiki/2011/b/b4/Lox71-rfp-lox-gfp_1.png" width="550px"/>
</li>
</li>
</ul>
</ul>
<p>
<p>
-
The <i>in vitro</i> assay with K649200 was made in advance. The preexperiment allowed  
+
The <i>in vitro</i> assay with K649200 was made in advance. The preliminary experiment allowed  
-
us to confirm that the Cre-mediated recombination on lox2272 cassette works as designed.  
+
us to confirm that the Cre-mediated recombination on <i>lox2272</i> cassette works as designed.  
In the assay, Cre recombinase was added to the linear DNA and incubated for 0.5, 2, and 4 hours.   
In the assay, Cre recombinase was added to the linear DNA and incubated for 0.5, 2, and 4 hours.   
Images of the experiments have been added below.
Images of the experiments have been added below.
Line 813: Line 808:
When checking the result by electrophoresis, there were several bands in samples to  
When checking the result by electrophoresis, there were several bands in samples to  
which Cre was added(1st, 2nd lane from right which corresponds to 4 hr and 2 hr respectively).  
which Cre was added(1st, 2nd lane from right which corresponds to 4 hr and 2 hr respectively).  
-
It indicates that excision of the lox sites successfully occurred.  
+
It indicates that excision of the <i>lox</i> sites successfully occurred.  
To know detailed about this assay, please see here,  
To know detailed about this assay, please see here,  
-
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#7."><i>in vitro</i> assay for lox2272</a>
+
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#7."><i>in vitro</i> assay for <i>lox2272</i></a>
</p>
</p>
Line 833: Line 828:
<tr>
<tr>
<td>1</td>
<td>1</td>
-
<td>PlacIQ-lox-RFP-lox-GFP(pSB3K3)<br />P<sub>BAD</sub>/araC-Cre(pSB1A2)</td>
+
<td>PlacIQ-<i>lox</i>-<span class="gene">rfp</span>-<i>lox</i>-<span class="gene">gfp</span>(pSB3K3)<br />P<sub>BAD</sub>/araC-Cre(pSB1A2)</td>
<td style="text-align:center;">+</td>
<td style="text-align:center;">+</td>
</tr>
</tr>
<tr>
<tr>
<td>2</td>
<td>2</td>
-
<td>PlacIQ-lox-RFP-lox-GFP(pSB3K3)<br />P<aub>BAD</aub>/araC-Cre(pSB1A2)</td>
+
<td>PlacIQ-<i>lox</i>-<span class="gene">rfp</span>-<i>lox</i>-<span class="gene">gfp</span>(pSB3K3)<br />P<sub>BAD</sub>/araC-Cre(pSB1A2)</td>
<td style="text-align:center;">-</td>
<td style="text-align:center;">-</td>
</tr>
</tr>
<tr>
<tr>
<td>3</td>
<td>3</td>
-
<td>PlacIQ-lox-RFP-lox-GFP(pSB3K3)<br /> : negative control </td>
+
<td>PlacIQ-<i>lox</i>-<span class="gene">rfp</span>-<i>lox</i>-<span class="gene">gfp</span>(pSB3K3)<br /> : negative control </td>
<td style="text-align:center;">+</td>
<td style="text-align:center;">+</td>
</tr>
</tr>
Line 855: Line 850:
and in each case the florescence levels were measured by flow cytometer and FLA.  
and in each case the florescence levels were measured by flow cytometer and FLA.  
To know the detailed method about this assay, please see here  
To know the detailed method about this assay, please see here  
-
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#8."><i>in vivo</i> assay for lox cassettes</a>.
+
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#8."><i>in vivo</i> assay for <i>lox</i> cassettes</a>.
</p>
</p>
-
<p>
+
-
We measured the fluorescence levels of two different constructions to prove
+
-
that recombination only occurs in presence of Cre recombinase. 
+
-
</p>
+
-
 
+
-
<div align="center">
+
-
<img src="https://static.igem.org/mediawiki/2011/a/a2/Flow_cytometer.png"/>
+
-
</div>
+
<p>
<p>
-
We also confirmed our results optically by taking florescence photographs.  
+
We confirmed our results optically by taking florescence images.  
-
Whole samples were plated and incubated in 37℃ for 12 hours.  
+
K649201 transformants with with 0.5 hr-induction of Cre in liquid medium and its two control strains were                   plated and incubated in 37&deg;C for 12 hours. Images of the three conditions were taken using red  
-
Photographs of three samples of K649201 were taken at 0.5 hours using red  
+
florescence filter, green florescence filter and no filter as shown below, respectively.
florescence filter, green florescence filter and no filter as shown below, respectively.
</p>
</p>
Line 890: Line 877:
<p>
<p>
-
Fig 1.Cre-meditated recombination at lox2272 cassette.  
+
Fig. 3.2 Cre-meditated recombination at <i>lox2272</i> cassette. Cre-induction period of 0.5 hr
-
Period of 0.5 hr. (a)The leftmost is a negative control which don't have Cre-expressing plasmid.  
+
                        (a)Overlay of Green and Red channel. The leftmost is a negative control which don't have Cre-expressing          
-
The center is an arabinose induced sample which has both Cre plasmid and BioBrick K649201.  
+
                        plasmid. The center is an arabinose induced sample which has both Cre plasmid and BioBrick K649201.  
The rightmost is a uninduced strain which has both plasmid like as the center.  
The rightmost is a uninduced strain which has both plasmid like as the center.  
-
Red florescence of three samples detected (b)Detection of GFP. The order of samples is same as above.  
+
(b)Detection of GFP. The order of samples is same as above.  
-
(c)Detection of mCherry Overlay. The order of samples is same as above.
+
(c)Detection of mCherry. The order of samples is same as above.
</p>
</p>
<p>
<p>
On the sample with the P<sub>BAD</sub>/araC-Cre construction, we found that recombination occurred  
On the sample with the P<sub>BAD</sub>/araC-Cre construction, we found that recombination occurred  
-
when arabinose was added. Opposite to this result, when we measured the levels of the sample  
+
when arabinose was added. In contrast to this result, when we measured the levels of the sample  
without the P<sub>BAD</sub>/araC-Cre construction, we found that the GFP levels were far lower than  
without the P<sub>BAD</sub>/araC-Cre construction, we found that the GFP levels were far lower than  
those of the sample with the P<sub>BAD</sub>/araC-Cre construction. This clearly proves that our  
those of the sample with the P<sub>BAD</sub>/araC-Cre construction. This clearly proves that our  
-
lox constructions, both in K649201 and K649202, respond correctly to the effects of Cre recombinase.  
+
<i>lox</i> constructions, both in K649201 and K649202, respond correctly to the effects of Cre recombinase.  
-
We could also observe recombination occurred when arabinose was not added, which can be explained  
+
A slight detection of green florescence in plate absence of P<sub>BAD</sub>/araC-Cre can be explained
-
due to a leaking in the P<sub>BAD</sub>/araC promoter.<br />The pictures of K649202 are on  
+
                        that there happened cross-talk to green channel by FMN(Flavin mononucleotide) or expression of GFP according
-
<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#8.">here</a>.
+
                        to malfunction of terminator before <span class="gene">gfp</span>. We could also observe recombination occurred when arabinose was not  
 +
                        added, which can be explained due to a leaking in the P<sub>BAD</sub>/araC promoter.You can find that K649202 also works well from the images of K649202 on<a href="https://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#8."> here</a>.
</p>
</p>
<p>
<p>
-
Furthermore, we confirmed the previous results of the flow cytometer measurements by observing that  
+
Furthermore, we could observe that the arabinose(+) sample of K649202 has higher green/red ratio than that of K649201, which implying the frequency of <i>lox71/66</i> casette is higher than that of <i>lox2272</i>.
-
the arabinose(+) sample of K649202 was brighter than that of K649201.
+
</p>
</p>
<div align="center">
<div align="center">
<img src="https://static.igem.org/mediawiki/2011/8/86/111001DK_30_eachpair_111003.png" /><br />
<img src="https://static.igem.org/mediawiki/2011/8/86/111001DK_30_eachpair_111003.png" /><br />
-
<span class="graph_title">>Fig 2. Photograps of six samples of K649202 (up) and K649201 (down) at period of 0.5 hr</span>
+
<span class="graph_title">Fig. 3.3 Image of six samples of K649201 (up) and K649202 (down) at period of 0.5 hr</span>
-
</div>
+
</div><br />
<table border="0">  
<table border="0">  
Line 928: Line 915:
<td><img src="https://static.igem.org/mediawiki/2011/archive/5/52/20111004160721%21Proportion_area.png" /></td>
<td><img src="https://static.igem.org/mediawiki/2011/archive/5/52/20111004160721%21Proportion_area.png" /></td>
<td>
<td>
-
Fig 3. identical plates with Fig 2.<br />
+
Fig. 3.4 identical plates with Fig. 3.3<br />
(a)expression levels of red and green florescence of K649201<br />
(a)expression levels of red and green florescence of K649201<br />
(b)expression levels of red and green florescence of K649202<br />
(b)expression levels of red and green florescence of K649202<br />
Line 942: Line 929:
<p>
<p>
As we examining green florescence in comparison to red florescence, green expression level was lower than red in  
As we examining green florescence in comparison to red florescence, green expression level was lower than red in  
-
K649201(Fig. 3(a)), which meaning that considerable cells didn’t undertake excision yet. In contrast, green  
+
K649201(Fig. 3.4(a)), which meaning that considerable plasmids in those cells yet. In contrast, green expression level exceeded red in K649202(Fig. 3.4(b)). This result implies that recombination frequency of  
-
expression level exceeded red in K649202(Fig. 3(b)). This result implies that recombination frequency of  
+
<i>lox71/66</i> cassette is relatively high than that of <i>lox2272</i> cassette.<br />
-
lox71/66 cassette is relatively high than that of lox2272 cassette.<br />
+
-
This result was true for all periods of time during the measurement (Fig#a through d),
+
-
which suggests that recombination frequency of lox71/66 is higher than that of lox2272 cassette.
+
</p>
</p>
-
 
+
<center><img src="https://static.igem.org/mediawiki/2011/a/a2/Flow_cytometer.png"/ width="500px" ></center><br>
 +
                <p>    <span class="graph_title">Fig. 3.5 Green fluorescence level of each cell was detected by flow cytometer.<br>
 +
                        (a)arabinose induced strain containing only K649201 and cre-expressing plasmid (b)arabinose supplied strain containing only K649201 (c)arabinose induced starin containing K649202 and cre-expressing plasmid (d)arabinose supplied strain containing only K649202<br>
 +
                </p>
 +
                <p>
 +
                The higher recombination efficiency of <i>lox71/66</i> compare to <i>lox2272</i> was confirmed also by flow cytometer intensity of <i>lox71/66</i> was higher than that of lox2272, which supports the result detected by FLA.
 +
                </span>
 +
                </p>
 +
<h4 id="3.2.4">3.2.4 Playing Fair: Future Work</h4>
<h4 id="3.2.4">3.2.4 Playing Fair: Future Work</h4>
<p>
<p>
-
To make each of the outcomes (R, P, and S) equally probable, we are going to examine the recombination  
+
To make each of the outcomes (R, P, and S) equally probable, we are going to quantify the recombination frequency of each lox cassette. This information and adequate Cre induction will be likely to allow us to have an RPS player  
-
frequency of each lox cassette. This will be likely to allow us to have an RPS player  
+
<span class="name">E. coli</span> whose choice of either of rock, paper or scissors cannot be predicted.
<span class="name">E. coli</span> whose choice of either of rock, paper or scissors cannot be predicted.
</p>
</p>
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/9/96/Image150.jpg" />
+
<img src="https://static.igem.org/mediawiki/2011/e/e6/Regulating_time_1.png" width="700px"/>
</div>
</div>
Line 971: Line 963:
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/2/28/Image042.png" />
+
<img src="https://static.igem.org/mediawiki/2011/2/28/Image042.png" width="500px" />
</div>
</div>
                
                
-
<h4 id="3.3.1">3.3.1 Introduction: Minimal differences determine who will survive</h4>
+
<h4 id="3.3.1">3.3.1 Introduction: Very small differences determine who will survive</h4>
<p>
<p>
In this section we will show a shocking scenario of evolution:  
In this section we will show a shocking scenario of evolution:  
the future of each of three different rival strains (whether the strain will die or survive)  
the future of each of three different rival strains (whether the strain will die or survive)  
-
is marked by minimal differences between the initial population densities of the strains.  
+
is marked by very small differences between the initial population densities of the strains (a phenomenon also known as the &ldquo;butterfly effect&rdquo;).  
Furthermore, we will also show that we can apply this very interesting result to create a randomizer  
Furthermore, we will also show that we can apply this very interesting result to create a randomizer  
that can be used in our Rock-Paper-Scissors game, due to the fact that only one of the rival strains  
that can be used in our Rock-Paper-Scissors game, due to the fact that only one of the rival strains  
will survive. More specifically, we assign to each of the three rival strains either of Rock, Paper or Scissors,  
will survive. More specifically, we assign to each of the three rival strains either of Rock, Paper or Scissors,  
-
make them compete for survival and take the surviving strain to represent the bacteria’s choice for the RPS game.
+
make them compete for survival and take the surviving strain to represent the bacteria's choice for the RPS game.
</p>
</p>
                
                
Line 990: Line 982:
<p>
<p>
The idea for creating this randomizer was born from a paper written in  
The idea for creating this randomizer was born from a paper written in  
-
1996 by Durret and Levin. In it, the authors described a system of three types of bacteria that competed for  
+
1996 by Durrett and Levin. In it, the authors described a system of three types of bacteria that competed for  
survival in dynamic that resembled a Rock-Paper-Scissors (RPS) game.  
survival in dynamic that resembled a Rock-Paper-Scissors (RPS) game.  
However, the model proposed in this paper is not fully appropriate for our RPS randomizer,  
However, the model proposed in this paper is not fully appropriate for our RPS randomizer,  
Line 1,016: Line 1,008:
<div align="center">
<div align="center">
-
<img src="https://static.igem.org/mediawiki/2011/b/bf/Image044.png" />
+
<img src="https://static.igem.org/mediawiki/2011/b/bf/Image044.png" width="500px" />
</div>
</div>
          
          
Line 1,037: Line 1,029:
<p>
<p>
-
In the model described by Durret and Levin’s paper the equations were as follows:
+
In the model described by Durrett and Levin’s paper the equations were as follows:
</p>
</p>
Line 1,056: Line 1,048:
</p>
</p>
<p>
<p>
-
Now, setting the parameters as follows, the graph below was created by Durret and Levin.
+
Now, setting the parameters as follows, the graph below was created by Durrett and Levin.
</p>
</p>
Line 1,070: Line 1,062:
<h4 id="3.3.5">3.3.5 Our New Model</h4>
<h4 id="3.3.5">3.3.5 Our New Model</h4>
<p>
<p>
-
As mentioned before, the model proposed by Durret and Levin has critical limitations as a randomizer for the RPS game.  
+
As mentioned before, the model proposed by Durrett and Levin has critical limitations as a randomizer for the RPS game.  
To be able to create a true randomizer, we modified the differential equations of the model taking care to give it  
To be able to create a true randomizer, we modified the differential equations of the model taking care to give it  
a biological meaning. With our new differential equations, any of the three types of bacteria can ultimately survive  
a biological meaning. With our new differential equations, any of the three types of bacteria can ultimately survive  
Line 1,080: Line 1,072:
randomizer because of the imprecisions in the measurements that result, for example, when using micropipettes.  
randomizer because of the imprecisions in the measurements that result, for example, when using micropipettes.  
This randomizer describes a new competition dynamic that could not be reproduced in the previous model proposed  
This randomizer describes a new competition dynamic that could not be reproduced in the previous model proposed  
-
by Durret and Levin due to the instability along the
+
by Durrett and Levin due to the instability along the
<img src="https://static.igem.org/mediawiki/2011/e/e0/Image088.png" alt="u1">axis.
<img src="https://static.igem.org/mediawiki/2011/e/e0/Image088.png" alt="u1">axis.
</p>
</p>
Line 1,098: Line 1,090:
and we graph this equations using a Matlab program,  
and we graph this equations using a Matlab program,  
we get a graph which clearly shows there are stable points on each of the three axes  
we get a graph which clearly shows there are stable points on each of the three axes  
-
(Figure 1, left).
+
(Fig. 1, Up).
</p>
</p>
Line 1,107: Line 1,099:
<div align="center">
<div align="center">
-
Figure 1. Up: Our New model. Down: The Old Model
+
Fig. 1 Up: Our New model. Down: The Old Model
</div>
</div>
<p>
<p>
-
These stable points (u1,0,0), (0,u2,0) and (0,0,u3) indicate that for the equations  
+
These stable points (u<sub>1</sub>,0,0), (0,u<sub>2</sub>,0) and (0,0,u<sub>3</sub>) indicate that for the equations  
we have set all of the three strains may ultimately survive for infinite peiriods of time.  
we have set all of the three strains may ultimately survive for infinite peiriods of time.  
-
The differences between our model and the model of Durret and Levin can be seen graphically  
+
The differences between our model and the model of Durrett and Levin can be seen graphically  
-
in Figure 1. These graphs were plotted using Matlab.  
+
in Fig. 1. These graphs were plotted using Matlab.  
</p>
</p>
<p>
<p>
Note that the parameters we have set for our equations satisfy the initail conditions  
Note that the parameters we have set for our equations satisfy the initail conditions  
-
of the model proposed by Durret and Levin (indicated in black font)  
+
of the model proposed by Durrett and Levin (indicated in black font)  
<img src="https://static.igem.org/mediawiki/2011/a/a4/Colimodel4.png" alt="new terms" width="800px"/>
<img src="https://static.igem.org/mediawiki/2011/a/a4/Colimodel4.png" alt="new terms" width="800px"/>
</p>
</p>
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<p>
<p>
-
From the graph of our new model (Figure 1, left) it can be deduced that there are paths  
+
From the graph of our new model (Fig. 1, left) it can be deduced that there are paths  
-
that converge at stable points (u1,0,0), (0,u2,0) and (0,0,u3), and that this paths all  
+
that converge at stable points (u<sub>1</sub>,0,0), (0,u<sub>2</sub>,0) and (0,0,u<sub>3</sub>), and that this paths all  
have an approximately common origin. In this section we would like to show that the  
have an approximately common origin. In this section we would like to show that the  
origin of these paths is practically the same, and that in that sense we have designed  
origin of these paths is practically the same, and that in that sense we have designed  
Line 1,148: Line 1,140:
<p>
<p>
In the following set of graphs we will make it obvious that each of the three  
In the following set of graphs we will make it obvious that each of the three  
-
different strains of E. coli to survive in a random fashion by minimal
+
different strains of E. coli to survive in a random fashion by very small
differences on the initial concentrations of each strain.
differences on the initial concentrations of each strain.
</p>
</p>
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</td>
</td>
<td rowspan="2">
<td rowspan="2">
-
We this graphs it becomes clear that the imprecisions in experimental measurements  
+
With these graphs it becomes clear that the imprecisions in experimental measurements  
(i.e. pipetting) are enough to cause the outcome of Rock, Paper or Scissors signaling  
(i.e. pipetting) are enough to cause the outcome of Rock, Paper or Scissors signaling  
molecule to be random. Consequently, we can conclude that this randomizer is not  
molecule to be random. Consequently, we can conclude that this randomizer is not  
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</tr>
</tr>
</table>
</table>
 +
 +
<h2>References</h2>
 +
<p>
 +
<ul>
 +
<li>Patrick C. Seed <i>et al</i>. &ldquo;Activation of the Pseudomonas aeruginosa lasI Gene by LasR and the Pseudomonas Autoinducer PAI: an Autoinduction Regulatory Hierarchy&rdquo; JOURNAL OF BACTERIOLOGY (1995)</li>
 +
<li>Shotaro Ayukawa <i>et al</i>. &ldquo;Construction of a genetic AND gate under a new standard for assembly of genetic parts&rdquo; BMC Genomics (2010)</li>
 +
<li>Robert Sidney Cox, III <i>et al</i>. &ldquo;Programming gene expression with combinatorial promoters&rdquo; molecular system biology (2007)</li>
 +
<li>Rolf Lutz <i>et al</i>. &ldquo;Independent and tight regulation of transcriptional units in Escherichia coli via the LacR/O, the TetR/O and AraC/I1-I2 regulatory elements&rdquo; Nucleic Acids Research (1997)</li>
 +
<li>Karina B.Xavier and Bonnie L.Bassler 2004. Regulation of Uptake and Processing of the Quorum-Sensing Autoinducer AI2 in Escherichia coli. JOURNAL OF BACTERIOLOGY, Jan. 2005, p. 238-248</li>
 +
<li>Ting Xue, Liping Zhao, Haipeng Sun, Xianxuan Zhou, Baolon Sun 2009. LsrR-binding site recognition and regulatory characteristics in Escherichia coli AI-2 quorum sensing. Cell Research (2009), p.1258-1268</li>
 +
<li>Liang Wang, Yoshifumi Hashimoto, Chen-Yu Tsao, James J.Valdes, and William E.Bentley 2004. Cyclic AMP(cAMP) and cAMP Receptor Protein Influence both Synthesis and Uptake of Extracellular Autoinducer 2 in Escherichia coli. JOURNAL OF BACTERIOLOGY, Mar. 2005, p. 2066-2076</li>
 +
<li>Jean Livet, Tamily A. Weissman, Hyuno Kang, Ryan W. Draft, Ju Lu, Robyn A. Bennis, Joshua R. Sanes and Jeff W. Lichtman (2007). Transgenic strategies for combinatorial expression of fluorescent proteins in the nervous system. Nature.</li>
 +
<li>Kimi Araki, Masatake Araki1 and Ken-ichi Yamamura (2002). Site-directed integration of the cre gene mediated by Cre recombinase using a combination of mutant <i>lox</i> sites, Nucleic Acids Research</li>
 +
<li>Durrett, R., Levin, S. Allelopathy in Spatially Distributed Populations (1997). Journal of Theoretical Biology, 185, 165-171. </li>
 +
 +
</ul>
 +
</p>

Latest revision as of 03:06, 29 October 2011

Tokyo Tech 2011

Rock-Paper-Scissors game

Introduction

The Hands

The first step towards making an RPS game that can be played between humans and bacteria is giving each player a set of signaling molecules through which they can communicate their choice of rock, paper or scissors. For that purpose we created two sets of three signaling molecules corresponding each to rock, paper or scissors. For humans we used IPTG, aTc and salicylate, respectively. For E. coli we used 3OC6-HSL, 3OC12-HSL and AI-2, respectively.


The Judges

Although we defined a set of six signaling molecules that can be used to play the RPS game, we still need to find a way to know who wins the game. To know who the winner of each game is, we designed a set of E. coli that act as judges. Because there were no working parts related to AI-2 or 3OC12-HSL, we constructed new working lasI promoter, lsrA promoter and LsrR coding gene.


The Randomizers

Although our set of six signaling molecules allows us to play RPS with E. coli, we must make sure E. coli can choose any of its three signaling molecules with the same probability in order to be able to play RPS fairly and properly. To do so, we designed three kinds of randomizers.

1. The Hands

The first step towards making an RPS game that can be played between humans and bacteria is giving each player a set of signaling molecules through which they can communicate their choice of rock, paper or scissors. For that purpose we created two sets of three signaling molecules corresponding each to rock, paper or scissors. For humans we used IPTG, aTc and salicylate, respectively. For E. coli we used 3OC6-HSL, 3OC12-HSL and AI-2, respectively.

2. The Judges

the Judge

Although we defined a set of six signaling molecules that can be used to play the RPS game, we still need to find a way to know who wins the game. To know who the winner of each game is, we designed a set of E. coli that act as judges. Each Judge E. coli has an AND-gate promoter and a fluorescent protein gene that is expressed when the AND-gate promoter is activated. In this way, the Judge E. coli can let us know its decision by producing GFP, RFP or CFP to indicate whether humans win, lose or it is a tie, respectively.

2.1 Using AND-Gate promoters to create Judges

The first step to make the Judge E. coli was to find a logic device which could allow the Judge to decide who the winner of the RPS game was. We found that the AND-gate promoters would fit perfectly for that purpose, since they can take two signaling molecules as inputs and produce one indicator as output. Since each of the players has a set of three different signaling molecules, we need a set of nine Judges, each of which has an AND-gate promoter that is activated only by one of the nine possible pairs of signaling molecules. These combinations are shown in the image below.

Our next mission was then to check if there were AND-gate promoters BioBricks that we could use. We searched in the Registry and found a potential AND-gate promoter designed by iGEM 2007's team Tokyo_Tech. This potential AND-gate promoter is designed to be activated by the addition of both IPTG and 3OC6-HSL. However, there was no data showing the IPTG dependency of this promoter, so we did experiments and confirmed this dependency for the first time in iGEM. We concluded that the addition of both IPTG and 3OC6-HSL regulates the activity of this AND-gate promoter. In this way, we completed the construction of one of the Judges E. coli, which proves in principle that our game is feasible. To know the detailed method about this assay, please see here.


Fig. 2.1 Tokyo_Tech AND-gate promoter

This Plux-lac hybrid promoter contains two LacI operators, a LuxR operator and luxR. We introduced this part into LacI expressing E. coli strain. Because IPTG controls the binding of LacI to two LacI-operator parts and 3OC6-HSL controls the binding of LuxR to a LuxR-operator part, the gfp gene activity of the reporter part is dually regulated by IPTG and 3OC6-HSL. We used promoterless pSB3K3-gfp (BBa_J54103) as a negative control, and pAC-Pλ-gfp (chloramphenicol-resistance), which constitutively expressed GFP, as a positive control. To know about the mechanism of this promoter click here.

2.2 Creating Parts that responded correctly to our set of Signaling Molecules

In the process of constructing enough AND-gates that could suffice the needs of our RPS game design, we discovered two faulty BioBricks: lsrA promoter (BBa_K117002) and las promoter (BBa_J64010). Because of these faulty parts, the Judge E. coli set we had designed could only sense the Player E. coli's signaling molecule 3OC6-HSL (Rock). This ultimately led to an unfair game because humans could win every time they played with the Paper signaling molecule (for more on the “Sad story of the Rock Player” click here).

To fix this problem, we improved the old defective las and lsrA promoters parts by making new parts that work! As can be seen in the experimental information below (see “Improving lsrA promoter” and “Improving las promoter”), we confirmed our lasI promoter (BBa_K649000) and lsrA promoter (BBa_K649100) work perfectly!

Since the lsrA promoter plays a key role in the correct functioning of AI-2, fixing these parts now allows us to use AI-2 as a signaling molecule, which is a promising advance because of the characteristics of the AI-2 mechanism. This mechanism prevents AI-2 from cross-talking with other signaling molecules such as AHL. Hence, this signaling molecule is a very powerful tool to build complex Synthetic Biology systems.

Finally, one thing we would like outline is that although the promoters we made are single input promoters, confirmation of their activity is required as a reference to construct AND gate promoters. Therefore, we solved important issues and made significant advances towards constructing AND-gate promoters. This allows E. coli to also choose the signaling molecules corresponding to Paper and Scissors, so we have again a working RPS game design.

2.3 Improving PlsrA

activity
Fig. 2.2 Not working lsrA promoter(BBa_K117002)
activity and our new lsrA promoter(BBa_K649104)
activity

We confirmed that the lsrA promoter (BBa_K117002) does not work properly (samples used our experiment are listed in Table 2.1 below). The fluorescence intensity of GFP of lsrA promoter-gfp((BBa_K117002)-gfp) was lower even than those of the negative control (Fig. 2.2), which clearly shows that lsrA promoter((BBa_K117002) does not work as expected. In this experiment, we measured transcriptional activity of lsrA promoter by introducing a gfp gene downstream of this promoter (Fig. 2.3).

Table 2.1 Samples used our experiment
Name Strain Plasmid
sample1 JD22597 Ptet-gfp on pSB1A2
sample2 Promoterless-gfp on pSB6A1
sample3 PlsrA-gfp on pSB1A2 (BBa_K649104)
sample4 PlsrA-gfp on pSB1A2 ((BBa_K117002)-gfp)
Fig2.3
Fig. 2.3 lsrA promoter-gfp((BBa_K117002)-gfp)

To solve this problem, we created the first working iGEM lsrA promoter (BBa_K649100). Its fluorescence intensity was much higher than that from a promoter-less gfp negative control plasmid, showing that our new lsrA promoter works(Fig. 2.5). In this experiment, we measured the transcriptional activity of our lsrA promoter by introducing a gfp gene downstream of the promoter(BBa_K649104, Fig. 2.4). Details about this experiment can be found here.

Fig2.4
Fig. 2.4 lsrA promoter-gfp(BBa_K649104)

Fig4
Fig. 2.5 LsrR represses lsrA promoter.

Moreover, this promoter can be repressed by our new LsrR part(BBa_K649105). (samples used our experiments are listed in Table 2.2 below) The fluorescence intensity of GFP of sample 3 was three times as large as that of sample 4. This result shows that LsrR successfully repressed lsrA promoter. In this experiment, we measured LsrR repression activity by introducing a gfp gene downstream of lsrA promoter ((BBa_K649105, Fig. 2.6). Details about this experiment can be found here.

Table2.2 Samples used our experiment
Name Strain Plasmid
sample1 JM2.300 Ptet-gfp on pSB6A1
sample2 Promoterless-gfp on pSB3K3
sample3 MG1655 PlsrA-gfp on pSB3K3
sample4 PlsrA-gfp-PlsrR-lsrR on pSB3K3
Fig.5
Fig. 2.6 lsrA promoter-gfp-lsrR promoter-lsrR(BBa_K649105)

2.4 Improving las promoter

Fig. 2.7 (a) (b)

Fig. 2.7 (a): Not working lasI promoter (BBa_J64010). Fig. 2.7 (b): New working lasI promoter (BBa_K649000) we made. We confirmed it works as expected. In our assay, we used the same LasR regulator part used in the assay of BBa_ J64010. Clearly, for our part the fluorescence intensity of 3OC12-HSL+ was higher than that of 3OC12-HSL-.
To know detailed methods about these lasI promoter assay, please see here, previous part and new part.

To prove that the LasR regulator used in our PlasI assay works, we did another assay. Details about this assay can be found here.

3. The Randomizers

Although our set of six signaling molecules allows us to play RPS with E. coli, we must make sure E. coli can choose any of its three signaling molecules with the same probability in order to be able to play RPS fairly and properly. To do so, we designed three kinds of randomizers: one kind which needs of three types of bacteria (each of which produces one of the three RPS signaling molecules), and the other kind that needs of only one type of bacteria which can synthetize each of the three signaling molecules one at a time and randomly. Namely, the randomizers are Single Colony Isolation, Survival of one Strain and Conditional Knockout by Recombination.

3.1 Single Colony Isolation

This is our simplest randomizer design. To make sure E. coli chooses any of its signaling molecules with equal probability, we put the constructs for each molecule inside a different bacterium, so we create three types of bacteria: one synthetizing the corresponding signaling molecule for rock, other synthetizing the corresponding signaling molecule for paper, and lastly one synthetizing the corresponding signaling molecule for scissors. By randomly isolating a single colony out of the many colonies that result from the mixing between the three types of E. coli, we get a random output as E. coli's choice for the RPS game.

3.2 Conditional Knockout by Recombination

Our second randomizer differs from our other two randomizers in that all the three signaling molecules are produced one at a time and randomly by only one type of bacteria. We were inspired by a paper about “brainbow” research on mice to create this randomizer (Livet J et al., 2007), which is based on the recombination mechanism of the enzyme Cre and the lox sequences. We designed a Cre-Lox system which allows E. coli to express one of its three signaling molecules by means of conditional knockout. The design is depicted in Fig. 1. It should be noted this randomizer is designed to be used at a single-cell level. When this randomizer is used in groups of cells, the different signals released by the cells will mix. In this case, by using microfluidic devices or isolating single colony of bacteria, we can obtain only one of the signaling molecules produced by the initial group of cells.

Fig. 3.1 - (a) Cre recombinase construction. (b) lox cassettes distribution for the randomizer design

3.2.1 The Requirements

Basically, each pair of lox sites (indicated by the same color) mark the points which the enzyme Cre will excise (they will be cut off the backbone along with the sequence between them). For a design that allows choosing randomly one of E. coli’s three signaling molecules, at least two cassettes of lox sites are needed. When these two cassettes of lox sites and protein coding sequences are arranged as in Fig. 3.1(b), only one signaling molecule is produced.

Our design also required a way to control luxI gene's expression. To do so, we used an inducible promoter instead of a constitutive promoter. A constitutive promoter would have caused luxI gene to be expressed beforehand and could lead to an E. coli producing two signaling molecules at the same time (the equivalent of showing two hands in the RPS game). In contrast, the inducible promoter prevents a particular gene from expressing preferentially.

One last but not less important requirement for our randomizer is that it should express each of the three signals not only one at a time, but also with the same probability. This makes the game fair in the sense that E. coli’s choice in the RPS game is not predictable.

3.2.2 The Mechanism

When the blue cassette of Lox sites is excised (Fig. 3.1), the signaling molecule coded by lasI (3OC6-HSL) will be produced. Likewise, when the black Lox cassette is excised, the signaling molecule coded by luxS (AI-2) will be produced. On the other hand, a third possible outcome is that recombination does not take place. In this case, the signaling molecule coded by luxI (3OC6-HSL) will be produced. Also note that excision of one kind of lox cassette removes the remaining cassette, thereby preventing further recombination.

As mentioned before, one of the requirements for our randomizer was to have at least two lox cassettes. This prevents excision of lox sites from different cassettes (for example one blue lox site and one black lox site). Because the lox71-lox66 cassette and the lox2272-lox2272 cassette are incompatible (Zorana Carter and Daniela Delneri et al., Yeast 2010), we can use them to build our randomizer.

3.2.3 Testing the Lox Cassettes

As stated above, we need two lox cassettes of different recombination frequency for randomizer. Because there was no working lox parts in registry, we constructed three original BioBricks for testing whether lox2272 and lox71/66 cassettes work. For the convenience of testing, fluorescence expressing genes were used in place of signal molecular expressing genes in construction. After figuring out their working in vitro, we tested them in vivo by detecting red and green fluorescence through fluoro imager and flow cytometer. Furthermore, we compared the relative recombination frequency of two cassettes . Our lox Cassettes constructions were working properly, and their recombination frequency were different from each other.

The in vitro assay with K649200 was made in advance. The preliminary experiment allowed us to confirm that the Cre-mediated recombination on lox2272 cassette works as designed. In the assay, Cre recombinase was added to the linear DNA and incubated for 0.5, 2, and 4 hours. Images of the experiments have been added below.

When checking the result by electrophoresis, there were several bands in samples to which Cre was added(1st, 2nd lane from right which corresponds to 4 hr and 2 hr respectively). It indicates that excision of the lox sites successfully occurred. To know detailed about this assay, please see here, in vitro assay for lox2272

For the in vivo assay, by detecting fluorescenc levels of GFP and mCherry, we could determine whether recombination occured in K649201 and K649202 and compare relative recombination frequency between two of them. We prepared a competent cell JM2.300 into which PBAD/araC-Cre(pSB1A2, BBa_I718008) had been constructed. Subsequently, our BioBrick was constructed into the cell.

sample arabinose
1 PlacIQ-lox-rfp-lox-gfp(pSB3K3)
PBAD/araC-Cre(pSB1A2)
+
2 PlacIQ-lox-rfp-lox-gfp(pSB3K3)
PBAD/araC-Cre(pSB1A2)
-
3 PlacIQ-lox-rfp-lox-gfp(pSB3K3)
: negative control
+

The strain was grown in a 3 mL liquid culture, and 75 µL of 2 M arabinose was added to induce Cre expression. We used two controls for the experiment. One was the same strain without arabinose induction, and the other was JM2.300 strain which was induced by arabinose and had only our BioBrick. All the strains were cultured each for periods of 0.5, 1, 2, and 4 hours, and in each case the florescence levels were measured by flow cytometer and FLA. To know the detailed method about this assay, please see here in vivo assay for lox cassettes.

We confirmed our results optically by taking florescence images. K649201 transformants with with 0.5 hr-induction of Cre in liquid medium and its two control strains were plated and incubated in 37°C for 12 hours. Images of the three conditions were taken using red florescence filter, green florescence filter and no filter as shown below, respectively.

(a)
(b)
(c)

Fig. 3.2 Cre-meditated recombination at lox2272 cassette. Cre-induction period of 0.5 hr (a)Overlay of Green and Red channel. The leftmost is a negative control which don't have Cre-expressing plasmid. The center is an arabinose induced sample which has both Cre plasmid and BioBrick K649201. The rightmost is a uninduced strain which has both plasmid like as the center. (b)Detection of GFP. The order of samples is same as above. (c)Detection of mCherry. The order of samples is same as above.

On the sample with the PBAD/araC-Cre construction, we found that recombination occurred when arabinose was added. In contrast to this result, when we measured the levels of the sample without the PBAD/araC-Cre construction, we found that the GFP levels were far lower than those of the sample with the PBAD/araC-Cre construction. This clearly proves that our lox constructions, both in K649201 and K649202, respond correctly to the effects of Cre recombinase. A slight detection of green florescence in plate absence of PBAD/araC-Cre can be explained that there happened cross-talk to green channel by FMN(Flavin mononucleotide) or expression of GFP according to malfunction of terminator before gfp. We could also observe recombination occurred when arabinose was not added, which can be explained due to a leaking in the PBAD/araC promoter.You can find that K649202 also works well from the images of K649202 on here.

Furthermore, we could observe that the arabinose(+) sample of K649202 has higher green/red ratio than that of K649201, which implying the frequency of lox71/66 casette is higher than that of lox2272.


Fig. 3.3 Image of six samples of K649201 (up) and K649202 (down) at period of 0.5 hr

(a) (b)
Fig. 3.4 identical plates with Fig. 3.3
(a)expression levels of red and green florescence of K649201
(b)expression levels of red and green florescence of K649202
(c)examined area for comparing between red and green florescence at each plate
(c)

As we examining green florescence in comparison to red florescence, green expression level was lower than red in K649201(Fig. 3.4(a)), which meaning that considerable plasmids in those cells yet. In contrast, green expression level exceeded red in K649202(Fig. 3.4(b)). This result implies that recombination frequency of lox71/66 cassette is relatively high than that of lox2272 cassette.


Fig. 3.5 Green fluorescence level of each cell was detected by flow cytometer.
(a)arabinose induced strain containing only K649201 and cre-expressing plasmid (b)arabinose supplied strain containing only K649201 (c)arabinose induced starin containing K649202 and cre-expressing plasmid (d)arabinose supplied strain containing only K649202

The higher recombination efficiency of lox71/66 compare to lox2272 was confirmed also by flow cytometer intensity of lox71/66 was higher than that of lox2272, which supports the result detected by FLA.

3.2.4 Playing Fair: Future Work

To make each of the outcomes (R, P, and S) equally probable, we are going to quantify the recombination frequency of each lox cassette. This information and adequate Cre induction will be likely to allow us to have an RPS player E. coli whose choice of either of rock, paper or scissors cannot be predicted.

In our next experiments, we are going to vary the reaction time and the distance between the lox sites of each cassette. We believe precise modification of this two parameters must lead to our goal of making a randomizer in which each of the signaling molecules can be expressed with the same frequency (which results in each of the outcomes being expressed with the same probability).

3.3 Survival of One strain

3.3.1 Introduction: Very small differences determine who will survive

In this section we will show a shocking scenario of evolution: the future of each of three different rival strains (whether the strain will die or survive) is marked by very small differences between the initial population densities of the strains (a phenomenon also known as the “butterfly effect”). Furthermore, we will also show that we can apply this very interesting result to create a randomizer that can be used in our Rock-Paper-Scissors game, due to the fact that only one of the rival strains will survive. More specifically, we assign to each of the three rival strains either of Rock, Paper or Scissors, make them compete for survival and take the surviving strain to represent the bacteria's choice for the RPS game.

3.3.2 Adjusting the Model to create a True Randomizer

The idea for creating this randomizer was born from a paper written in 1996 by Durrett and Levin. In it, the authors described a system of three types of bacteria that competed for survival in dynamic that resembled a Rock-Paper-Scissors (RPS) game. However, the model proposed in this paper is not fully appropriate for our RPS randomizer, since one of the three types of bacteria cannot ultimately survive (although it can dominate the system, i.e. have the highest population density, for definite periods of time). We will discuss more on the limitations we found in this model to be adopted as a randomizer and the modifications we made to create a true randomizer.

3.3.3 How the Three Types of Bacteria Compete for Survival

The three types of bacteria that compete for survival use three tactics to outcompete their rivals: the production of a toxin (a bacteriocin called colicin) that is toxic to other strains, resistance to the toxin produced by other strains, and a higher birth rate than their rival strains. Namely, the three types of bacteria are: colicin-producing E. coli (R), colicin-resistant E. coli (P) and colicin-sensitive E. coli (S). The colicin-producer outcompetes the colicin-sensitive by producing the colicin. The colicin-sensitive bacteria outcompetes the colicin-resistant because its birth rate is higher than that of the colicin-resistant. The colicin-resistant outcompetes the colicin producer because its birth rate is higher than that of the colicin producer. The colicin resistant bacteria are also able to produce colicin, but at a lower energetic cost, which allows them to have a higher birth rate.

The system was described by the following general differential equations

Where

3.3.4 The Old Model

In the model described by Durrett and Levin’s paper the equations were as follows:

Producer


Resistant


Sensitive


These equations show that the colicin-resistant bacteria are completely immune to colicin (there is not death factor associated to colicin in the equation for du2/dt). However, as will be explained afterwards, this results in a loss of balance that does not allow building a true randomizing system.

Now, setting the parameters as follows, the graph below was created by Durrett and Levin.





3.3.5 Our New Model

As mentioned before, the model proposed by Durrett and Levin has critical limitations as a randomizer for the RPS game. To be able to create a true randomizer, we modified the differential equations of the model taking care to give it a biological meaning. With our new differential equations, any of the three types of bacteria can ultimately survive by outcompeting the other two strains, which will die. More specifically, we limited the resistance of the colicin-resistant bacteria in the sense that it would produce a type of bacteriocin that is only toxic to itself and to the sensitive strain, and additionally the resistant strain would also be vulnerable to the colicin produced by the colicin-producer. Since which strain will be the one that survives is determined by very small differences in the initial concentrations of the three different populations of bacteria, in practice this systems becomes a randomizer because of the imprecisions in the measurements that result, for example, when using micropipettes. This randomizer describes a new competition dynamic that could not be reproduced in the previous model proposed by Durrett and Levin due to the instability along the u1axis.

our new model

If we set the parameters as follows

new model's coefficient

and we graph this equations using a Matlab program, we get a graph which clearly shows there are stable points on each of the three axes (Fig. 1, Up).


Fig. 1 Up: Our New model. Down: The Old Model

These stable points (u1,0,0), (0,u2,0) and (0,0,u3) indicate that for the equations we have set all of the three strains may ultimately survive for infinite peiriods of time. The differences between our model and the model of Durrett and Levin can be seen graphically in Fig. 1. These graphs were plotted using Matlab.

Note that the parameters we have set for our equations satisfy the initail conditions of the model proposed by Durrett and Levin (indicated in black font) new terms

3.3.6 The Biological Meaning of our Model

From a biological perspective, our model describes the existence of two strains of bacteria that produce two different types of bacteriocins. One of these strains is not completely resistant to its own bacteriocin nor to the bacteriocin produced by its rival strain. This can be justified as the consequence of insufficient/ineffective resistance protein production by the “resistant” strain. This limitation in the production of resistance protein could be thought of as a consequence of the “resistant” strain being a mutant of a colicin-sensitive strain.

3.3.7 Making it Obvious

From the graph of our new model (Fig. 1, left) it can be deduced that there are paths that converge at stable points (u1,0,0), (0,u2,0) and (0,0,u3), and that this paths all have an approximately common origin. In this section we would like to show that the origin of these paths is practically the same, and that in that sense we have designed a true randomizer (since, as mentioned before, the imprecisions that result in the experimental measurements will make it impossible to make the initial population density of the three strains the same).

In the following set of graphs we will make it obvious that each of the three different strains of E. coli to survive in a random fashion by very small differences on the initial concentrations of each strain.

We modeled our results using Matlab. As can be seen in the graphs below, each of the strains can survive if their initial density in only tree hundredths (a.u.) greater than the other two strains' initial concentrations.

output1 output2
coefficient of output1 coefficient of output2
output3 With these graphs it becomes clear that the imprecisions in experimental measurements (i.e. pipetting) are enough to cause the outcome of Rock, Paper or Scissors signaling molecule to be random. Consequently, we can conclude that this randomizer is not only feasible but also practical and effective (let alone interesting).
coefficient of output3

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