Difference between revisions of "Team:Peking/Improve"

 
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                 <div class="twelve columns centered text-center">
 
                 <div class="twelve columns centered text-center">
 
                     <h1>Improvement</h1>
 
                     <h1>Improvement</h1>
                    <p class="title1" style="text-align:center">In this section, you could see the Improvement.</p>
+
                 
 
                 </div>
 
                 </div>
 
             </div>
 
             </div>
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                             <div id="page-wrap">
 
                             <div id="page-wrap">
 
                                 <div id="sidebar" style="color:#000000">
 
                                 <div id="sidebar" style="color:#000000">
                                     <h4><a href="javascript:void(0);" onclick="naver('A')">Overview</a></h4>
+
                                     <h4><a href="javascript:void(0);" onclick="naver('A')">&bull;Fused&nbsp;with&nbsp;yEGFP</a></h4>
                                    <h4><a href="javascript:void(0);" onclick="naver('B')">Phase&nbsp;Separation</a></h4>
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                                     <h4><a href="javascript:void(0);" onclick="naver('B')">&bull;Phase&nbsp;Separation</a></h4>
                                    <ul>
+
                   
                                        <li><a href="javascript:void(0);" onclick="naver('B1')">Spontaneous</a></li>
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                                        <li><a href="javascript:void(0);" onclick="naver('B2')">The&nbsp;formation</a></li>
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                                    </ul>
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                                     <h4><a href="javascript:void(0);" onclick="naver('C')">Functional&nbsp;Organelles</a></h4>
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                                    <h4><a href="javascript:void(0);" onclick="naver('D')">Perspective</a></h4>
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                                 </div>
 
                                 </div>
 
                             </div>
 
                             </div>
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                                 <div class="content">
 
                                 <div class="content">
                                     <p>We fused part Frb<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209496) </a> and FKBP<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209023) </a>with yEGFP, which made it visible in the yeast under fluorescent microscope. Then we got part Frb-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601007"> (BBa_K2601007) </a> and FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601008"> (BBa_K2601008) </a>.</p>
+
                                     <p>We fused part Frb<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209496) </a> and FKBP<a href="http://parts.igem.org/Part:BBa_K209023"> (BBa_K209023) </a>with yEGFP, which made it visible in the yeast under fluorescent microscope. Then we got part Frb-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601007"> (BBa_K2601007) </a> and FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601008"> (BBa_K2601008) </a>.</p>
 
                                 </div>
 
                                 </div>
 
                             </div>
 
                             </div>
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TEF1-FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601026"> (BBa_K2601026) </a>;
 
TEF1-FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601026"> (BBa_K2601026) </a>;
 
<br/>
 
<br/>
PDH3-FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601027"> (BBa_K2601027) </a>. </p>
+
PDH3-FKBP-yEGFP<a href="http://parts.igem.org/Part:BBa_K2601027"> (BBa_K2601027) </a>.  
 +
</p>
 
<br/>
 
<br/>
 
<img src="https://static.igem.org/mediawiki/parts/f/f7/T--Peking--promoter-strength-new.png">
 
<img src="https://static.igem.org/mediawiki/parts/f/f7/T--Peking--promoter-strength-new.png">
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                                     <p></a></p><br/><br/><br/>       
 
                                     <p></a></p><br/><br/><br/>       
 
                                 </div>
 
                                 </div>
                            </div>
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           <div class="texttitle">Phase separation system
 
           <div class="texttitle">Phase separation system
<a id="A"></a></div>  
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<a id="B"></a></div>  
 
                             <hr style="border:2px dashed; height:2px" color="#666666">
 
                             <hr style="border:2px dashed; height:2px" color="#666666">
 
  <div class="coll">
 
  <div class="coll">
 
                                  
 
                                  
 
                                 <div class="content">
 
                                 <div class="content">
                                     <p>Moreover, we fused Frb-yEGFP with HOtag6 and FKBP-yEGFP with HOtag3. These parts can form phase separation in the presence of rapamycin (Fig. 2). The original part Frb<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209496) </a>and FKBP<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209023) </a>doesn't have this function.  
+
                                     <p>Moreover, we fused Frb-yEGFP with HOtag6 and FKBP-yEGFP with HOtag3. These parts can form phase separation in the presence of rapamycin (Fig. 2). The original part Frb<a href="http://parts.igem.org/Part:BBa_K209496"> (BBa_K209496) </a>and FKBP<a href="http://parts.igem.org/Part:BBa_K209023"> (BBa_K209023) </a>doesn't have this function.  
 
<br/>
 
<br/>
 
We uploaded 2 parts:
 
We uploaded 2 parts:
 
<br/>
 
<br/>
 
Frb-yEGFP-HOTag6<a href="http://parts.igem.org/Part:BBa_K2601010"> (BBa_K2601010) </a>;
 
Frb-yEGFP-HOTag6<a href="http://parts.igem.org/Part:BBa_K2601010"> (BBa_K2601010) </a>;
<a href="http://parts.igem.org/Part:BBa_K2601011">BBa_K2601011</a> ().
+
<br/>
 +
FKBP-yEGFP-HOTag3<a href="http://parts.igem.org/Part:BBa_K2601011"> (BBa_K2601011) </a>.
 
</p>
 
</p>
 
<br/>
 
<br/>
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Figure. 2  The improvement of Frb and FKBP fused with yEGFP.
 
Figure. 2  The improvement of Frb and FKBP fused with yEGFP.
 
<br/>
 
<br/>
(A) The structure of Frb and FKBP. Rapamycin induce the interaction between them.
+
Figure. 2A The structure of Frb and FKBP. Rapamycin induces the interaction between them.
 
<br/>
 
<br/>
(B) Design of RapaSPOT. FKBP is fused with mCherry and HOTag3 while Frb is fused with yEGFP and HOTag6. After adding rapamycin, they are expected to self-organize to form large assemblies, which will be an organelle in cells.
+
Figure. 2B Design of RapaSPOT. FKBP is fused with mCherry and HOTag3 while Frb is fused with yEGFP and HOTag6. After adding rapamycin, they are expected self-organizing to form large assemblies, which will be organelles in cells.
 
<br/>
 
<br/>
(C) Granules in chemical-induced SPOT after adding rapamycin. Ura3-FKBP-HOTag3(mCherry) and PDH3-Frb-HOTag6 with yEGFP are transferred and expressed in S. cerevisiae. Fluorescence images in both GFP and mCherry channels of cells are taken after the addition of 10 μM rapamycin. Granules occurs in less than 20 minutes and the two fluorescence channels merge well.<br/>
+
Figure. 2C Granules formed in chemical-induced SPOT after adding rapamycin. Ura3-FKBP-HOTag3 with mCherry and PDH3-Frb-HOTag6 with yEGFP are transferred and expressed in S. cerevisiae. Fluorescence images in both GFP and mCherry channels of cells are taken after adding 10 μM Figure. 2D Growth curves of wild-type yeast (black curve) and yeast strains of Ura3-FKBP-HOTag3 and PDH3-Frb-HOTag6 (red curve). They are measured after adding different concentration of rapamycin for 24 hours. Wild-type yeast cannot grow and reproduce normally while recombination yeast strains of FKBP-HOTag3 and Frb-HOTag6 can survive when exposed to rapamycin.
(D) Growth curves of wild-type yeasts (black curve) and yeast strains with Ura3-FKBP-HOTag3 and PDH3-Frb-HOTag6 (red curve). They are measured after adding different concentration of rapamycin for 24 hours. Wild-type yeasts cannot grow and reproduce normally while engineered yeasts with FKBP-HOTag3 and Frb-HOTag6 can survive when exposed to rapamycin.
+
 
<br/><br/><br/>
 
<br/><br/><br/>
 
<p>
 
<p>
Then, we drive the expression of Frb-yEGFP-HOTag6 with 3 promoters pUra3, pTEF1 and PDH3. As our <a href="https://2018.igem.org/Team:Peking/Model">Modeling</a> work predicts, the kinetics of a system depends on the concentration of the components and the interaction strength(Fig .3). We successfully uploaded 5 parts form them: <a href="http://parts.igem.org/Part:BBa_K2601032">BBa_K2601032</a> (pTet07-Frb-yEGFP-HOTag6), <a href="http://parts.igem.org/Part:BBa_K2601033">BBa_K2601033</a> (pTEF1-Frb-yEGFP-HOTag6), <a href="http://parts.igem.org/Part:BBa_K2601034">BBa_K2601034</a> (PDH3-Frb-yEGFP-HOTag6), <a href="http://parts.igem.org/Part:BBa_K2601011">BBa_K2601011</a> (pTEF1-FKBP-yEGFP-HOTag3) and <a href="http://parts.igem.org/Part:BBa_K2601011">BBa_K2601011</a> (PDH3-yEGFP-HOTag3).
+
Then we characterized the expression of Frb-yEGFP-HOTag6 with 3 promoters pUra3, pTEF1 and PDH3. As our <a href="https://2018.igem.org/Team:Peking/Model">Modeling</a> work predicts, the kinetics of a system depends on the concentration of the components and the interaction strength(Fig .3). We successfully uploaded 5 parts form them:  
 +
<br/>
 +
pTet07-Frb-yEGFP-HOTag6<a href="http://parts.igem.org/Part:BBa_K2601032"> (BBa_K2601032) </a>;
 +
<br/>
 +
pTEF1-Frb-yEGFP-HOTag6<a href="http://parts.igem.org/Part:BBa_K2601033"> (BBa_K2601033) </a>;
 +
<br/>
 +
PDH3-Frb-yEGFP-HOTag6<a href="http://parts.igem.org/Part:BBa_K2601034"> (BBa_K2601034) </a>;
 +
<br/>
 +
pTEF1-FKBP-yEGFP-HOTag3<a href="http://parts.igem.org/Part:BBa_K2601011"> (BBa_K2601011) </a>;
 +
<br/>
 +
PDH3-yEGFP-HOTag3<a href="http://parts.igem.org/Part:BBa_K2601011"> (BBa_K2601011) </a>.
 
</p>
 
</p>
  
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Figure. 3  The improvement of Frb and FKBP fused with yEGFP regulated by four kinds of promoters.  
 
Figure. 3  The improvement of Frb and FKBP fused with yEGFP regulated by four kinds of promoters.  
 
<br/>
 
<br/>
(A) The formation of SPOT can be described as a phase separation process of three components. Two important variable, the concentration of components and the interaction strength are marked in the figure.
+
Figure. 3A The formation of SPOT can be described as a phase separation process of three components. Two important variables, the concentration of components and the interaction strength are marked in the figure.
<br/>
+
(B) Flow Cytometry results of three promoters (Ura3, Tef2, and PDH3). The expression level of Ura3 is lowest while PDH3 is the strongest promoter.
+
 
<br/>
 
<br/>
(C) RapaSPOT of different promoter combinations after 10 μM rapamycin induction. Two axes stand for the expression level of components. After 3 hours, Only SPOT system with high level of Frb can be observed.
+
Figure. 3B Flow cytometry results of three promoters (pUra3, pTEF2, and PDH3). The expression level of Ura3 is the lowest while PDH3 is the strongest promoter.
 
<br/>
 
<br/>
(D) Proportion of yeasts with granules after rapamycin induction. The rapamycin is from 1μM to 100 μM.
+
Figure. 3C RapaSPOT of different promoter combinations after 10 μM rapamycin induction. Two axes stand for the expression level of components. After 3 hours, only SPOT system with high level of Frb can be observed.
 +
Figure. 3D Proportion of yeast with granules after rapamycin induction. The rapamycin concentration range is from 1μM to 100 μM.
 
</figcaption>
 
</figcaption>
  
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                     <ul class="copyright">
 
                     <ul class="copyright">
 
                         <!--<li>&copy; 2014 Sparrow</li> -->
 
                         <!--<li>&copy; 2014 Sparrow</li> -->
                         <li><a href="https://2018.igem.org/Team:Peking">Home</a>&nbsp;&nbsp;&nbsp;<a href="mailto:indigomad@pku.edu.cn">Contact</a></li>
+
                         <li><a href="https://2018.igem.org/Team:Peking">Home</a>&nbsp;&nbsp;&nbsp;<a href="mailto:pekingigem2018@126.com">Contact</a></li>
 
                         <span> &copy;2018 PEKING IGEM. All Rights Reserved.</span>
 
                         <span> &copy;2018 PEKING IGEM. All Rights Reserved.</span>
 
                         <li><a href="http://getbootstrap.com/2.3.2/">Based on Bootstrap</a></li>
 
                         <li><a href="http://getbootstrap.com/2.3.2/">Based on Bootstrap</a></li>

Latest revision as of 00:27, 18 October 2018

Improvement

Fused with yEGFP

We fused part Frb (BBa_K209496) and FKBP (BBa_K209023) with yEGFP, which made it visible in the yeast under fluorescent microscope. Then we got part Frb-yEGFP (BBa_K2601007) and FKBP-yEGFP (BBa_K2601008) .

Then we characterized the expression of Frb-yEGFP and FKBP-yEGFP with 4 promoters pUra3, pTet07, pTEF1 and PDH3. The expression of these promoters was measured through flow cytometry (Fig. 1).
We made these improved prats:
Tet07-Frb-yEGFP (BBa_K2601021) ;
PDH3-Frb-yEGFP (BBa_K2601023) ;
Tet07-FKBP-yEGFP (BBa_K2601025) ;
TEF1-FKBP-yEGFP (BBa_K2601026) ;
PDH3-FKBP-yEGFP (BBa_K2601027) .



Figure. 1 The strength of three different yeast promoters tested through flow cytometry.




Phase separation system

Moreover, we fused Frb-yEGFP with HOtag6 and FKBP-yEGFP with HOtag3. These parts can form phase separation in the presence of rapamycin (Fig. 2). The original part Frb (BBa_K209496) and FKBP (BBa_K209023) doesn't have this function.
We uploaded 2 parts:
Frb-yEGFP-HOTag6 (BBa_K2601010) ;
FKBP-yEGFP-HOTag3 (BBa_K2601011) .





Figure. 2 The improvement of Frb and FKBP fused with yEGFP.
Figure. 2A The structure of Frb and FKBP. Rapamycin induces the interaction between them.
Figure. 2B Design of RapaSPOT. FKBP is fused with mCherry and HOTag3 while Frb is fused with yEGFP and HOTag6. After adding rapamycin, they are expected self-organizing to form large assemblies, which will be organelles in cells.
Figure. 2C Granules formed in chemical-induced SPOT after adding rapamycin. Ura3-FKBP-HOTag3 with mCherry and PDH3-Frb-HOTag6 with yEGFP are transferred and expressed in S. cerevisiae. Fluorescence images in both GFP and mCherry channels of cells are taken after adding 10 μM Figure. 2D Growth curves of wild-type yeast (black curve) and yeast strains of Ura3-FKBP-HOTag3 and PDH3-Frb-HOTag6 (red curve). They are measured after adding different concentration of rapamycin for 24 hours. Wild-type yeast cannot grow and reproduce normally while recombination yeast strains of FKBP-HOTag3 and Frb-HOTag6 can survive when exposed to rapamycin.


Then we characterized the expression of Frb-yEGFP-HOTag6 with 3 promoters pUra3, pTEF1 and PDH3. As our Modeling work predicts, the kinetics of a system depends on the concentration of the components and the interaction strength(Fig .3). We successfully uploaded 5 parts form them:
pTet07-Frb-yEGFP-HOTag6 (BBa_K2601032) ;
pTEF1-Frb-yEGFP-HOTag6 (BBa_K2601033) ;
PDH3-Frb-yEGFP-HOTag6 (BBa_K2601034) ;
pTEF1-FKBP-yEGFP-HOTag3 (BBa_K2601011) ;
PDH3-yEGFP-HOTag3 (BBa_K2601011) .



Figure. 3 The improvement of Frb and FKBP fused with yEGFP regulated by four kinds of promoters.
Figure. 3A The formation of SPOT can be described as a phase separation process of three components. Two important variables, the concentration of components and the interaction strength are marked in the figure.
Figure. 3B Flow cytometry results of three promoters (pUra3, pTEF2, and PDH3). The expression level of Ura3 is the lowest while PDH3 is the strongest promoter.
Figure. 3C RapaSPOT of different promoter combinations after 10 μM rapamycin induction. Two axes stand for the expression level of components. After 3 hours, only SPOT system with high level of Frb can be observed. Figure. 3D Proportion of yeast with granules after rapamycin induction. The rapamycin concentration range is from 1μM to 100 μM.