Difference between revisions of "Team:Amoy/Notebook"

@@ Line 12: / Line 12: @@
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+<link rel="stylesheet" type="text/css" href="https://2015.igem.org/Template:Amoy/css/MenuCss?action=raw&amp;ctype=text/css" />
+<script type="text/javascript" src="https://2015.igem.org/Template:Amoy/Javascript/MenuJs?action=raw&amp;ctype=text/javascript"></script>
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 <body>
 <a style="width:50px; height:50px; position:fixed; right:30px; bottom:30px; z-index:9999; display:none; background:url(https://static.igem.org/mediawiki/2015/c/c1/Amoy-Home_Up_pic.gif) no-repeat center center #147abc;"  href="javascript:;" class="lanrenzhijia_top"></a>
@@ Line 75: / Line 78: @@
 <p class="detail_p">Extract plasmid from dry powder</br></p>
 <p class="detail_h1">Steps:</br></p>
-<p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
+<p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder.</br>
-. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
+. Suck 10μl of plasmid into 50μl of competent cell for transformation.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
 <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm</br>
+. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br>
-. Plasmid Extraction</br></p>
+. Plasmid extraction.</br></p>
 <p class="detail_h1">Product: </br></p>
-<p class="detail_p"> Plasmid of promote_J23100</br></p>
+<p class="detail_p"> Plasmid of promoter_J23100</br></br></br></p>
 </div>
 </div>
@@ Line 95: / Line 98: @@
 <p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/d/d9/Amoy-Notebook_node42-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/d/d9/Amoy-Notebook_node42-1.jpeg" />
 <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm</br>
+. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm.</br>
-. Plasmid Extraction</br></p>
+. Plasmid extraction.</br></p>
 <p class="detail_h1">Product:</br></p>
 <p class="detail_p">Plasmid of promoter_LacI</br></p>
@@ Line 113: / Line 116: @@
 <p class="detail_p">1. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e9/Amoy-Notebook_node43-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/6/64/Amoy-Notebook_node43-1.JPG" />
 <p class="detail_p"></br>3. Pick a single colony from the agar plate using a sterile pipette tip. </br>
 . Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm</br>
@@ Line 132: / Line 135: @@
 . Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/cd/Amoy-Notebook_node44-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/cd/Amoy-Notebook_node44-1.jpeg" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip.  </br>
@@ Line 152: / Line 155: @@
 . Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e4/Amoy-Notebook_node45-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e4/Amoy-Notebook_node45-1.jpeg" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
@@ Line 170: / Line 173: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Add 20μl ddH<sub>2</sub>O to solve the dry powder</br>
+. Add 20μL ddH<sub>2</sub>O to solve the dry powder.</br>
-. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
+. Suck 10μL of plasmid into 50μL of competent cell for transformation.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/41/Amoy-Notebook_node46-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/cf/Amoy-Notebook_node33-1.JPG" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm</br>
+. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br>
 . Plasmid Extraction</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> Plasmid of LacI_RBS_B0034</br></p>
+<p class="detail_p"> Plasmid of Plac_RBS_B0034</br></p>
 </div>
 </div>
@@ Line 190: / Line 193: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Add 20μl ddH<sub>2</sub>O to solve the dry powde</br>
+. Add 20μL ddH<sub>2</sub>O to solve the dry powder.</br>
-. Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
+. Suck 10μL of plasmid into 50μL of competent cell for transformation.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1a/Amoy-Notebook_node34-1.JPG" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm</br>
+. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br>
 . Plasmid Extraction</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> Plasmid of Promoter_J23100_RBS_B0030</br></p>
+<p class="detail_p"> Plasmid of P<sub>J23100</sub>_RBS_B0030</br></p>
 </div>
 </div>
@@ Line 212: / Line 215: @@
 . Add 20μl ddH<sub>2</sub>O to solve the dry powde</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/13/Amoy-Notebook_node48-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/d/d5/Amoy-Notebook_node48-1.JPG" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
@@ Line 232: / Line 235: @@
 . Add 20μl ddH<sub>2</sub>O to solve the dry powde</br>
 . Suck 10μl of plasmid into 50μl of competent cell for transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/5c/Amoy-Notebook_node49-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/5c/Amoy-Notebook_node49-1.jpeg" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip.  </br>
@@ Line 247: / Line 250: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">pcr amplification for gene ldh and double enzyme digestion</br></p>
+<p class="detail_p">PCR amplification for gene_<i>leudh</i> and double enzyme digestion</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. pcr amplification system for gene ldh</br></p>
+. PCR amplification system for gene_<i>leudh</i></br></p>
 <table class="col-md-12" style="margin-bottom: 50px;">
@@ Line 259: / Line 262: @@
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH20</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH<sub>2</sub>O</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 16μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">LDH-F</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"><i>leudh</i>-F</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1.5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">LDH-R</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"><i>leudh</i>-R</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1.5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">Pub18-LDH</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">pUB18-<i>leudh</i></td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1μL</td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">primestar</td>
+   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">Prime Star</td>
-   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> 20μL </td>
   </tr class="col-md-3">
 </table>
-<p class="detail_p">2. electrophoresis of PCR products of gene ldh</br>
+<p class="detail_p">2. Electrophoresis of PCR products of gene_<i>leudh</i></br>
-. Double enzyme digestion of gene ldh</br></p>
+. Double enzyme digestion of gene_<i>leudh</i></br></p>
 <table class="col-md-12" style="margin-bottom: 50px;">
   <tr style="border-bottom: 1px solid #aaaaaa; border-top: 1px solid #aaaaaa;">
-   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">item</td>
+   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">Components</td>
-   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa;" class="col-md-6">volume</td>
+   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa;" class="col-md-6">Volume</td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"> Gene </td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 20μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH2O</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH<sub>2<sub>O</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 20μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
    <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">buffer</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 10μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ErcoI</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">EcoR I</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">SpeI</td>
+   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">Spe I</td>
-   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> 5μL </td>
   </tr class="col-md-3">
 </table>
-<p class="detail_p">4. Cycle purity of digested gene ldh</br></p>
+<p class="detail_p">4. Cycle purity of digested gene_<i>leudh</i></br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> </br></p>
+<p class="detail_p"> Digested gene_<i>leudh</i> </br></p>
 </div>
 </div>
@@ Line 330: / Line 333: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">pcr amplification for gene fdh and double enzyme digestion</br></p>
+<p class="detail_p">PCR amplification for gene_<i>fdh</i> and double enzyme digestion</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. pcr amplification system for gene fdh</br></p>
+. PCR amplification system for gene_<i>fdh</i></br></p>
 <table class="col-md-12" style="margin-bottom: 50px;">
@@ Line 342: / Line 345: @@
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH20</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH<sub>2</sub>O</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 16μL</td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">FDH-F</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"><i>fdh</i>-F</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1.5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">FDH-R</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"><i>fdh</i>-R</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1.5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">Pub18-FDH</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">pUB18-<i>fdh</i></td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 1μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">primestar</td>
+   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">Prime Star</td>
-   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> 20μL </td>
   </tr class="col-md-3">
 </table>
-<p class="detail_p">2. electrophoresis of PCR products of gene fdh</br>
+<p class="detail_p">2. Electrophoresis of PCR products of gene_<i>fdh</i></br>
-. Double enzyme digestion of gene fdh</br></p>
+. Double enzyme digestion of gene_<i>fdh</i></br></p>
 <table class="col-md-12" style="margin-bottom: 50px;">
   <tr style="border-bottom: 1px solid #aaaaaa; border-top: 1px solid #aaaaaa;">
-   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">item</td>
+   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">Components</td>
-   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa;" class="col-md-6">volume</td>
+   <td style="padding-bottom: 10px; border-right: 1px solid #aaaaaa;" class="col-md-6">Volume</td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6"> Gene </td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 50μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH2O</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ddH<sub>2</sub>O</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6">10μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
    <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">buffer</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 10μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">ErcoI</td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa;" class="col-md-6">EcoR I</td>
-   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="padding-top: 15px; border-right: 1px solid #aaaaaa;" class="col-md-6"> 5μL </td>
   </tr>
   <tr style="border-bottom: 1px solid #aaaaaa;">
-   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">SpeI</td>
+   <td style="border-right: 1px solid #aaaaaa; border-left: 1px solid #aaaaaa; " class="col-md-6">Spe I</td>
-   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> </td>
+   <td style="border-right: 1px solid #aaaaaa;" class="col-md-6"> 5μL </td>
   </tr class="col-md-3">
 </table>
-<p class="detail_p">4. Cycle purity of digested gene fdh</br></p>
+<p class="detail_p">4. Cycle purity of digested gene_<i>fdh</i></br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> </br></p>
+<p class="detail_p"> Digested gene_<i>fdh</i></br></p>
 </div>
 </div>
@@ Line 413: / Line 416: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">Make connection of gene and terminator</br></p>
+<p class="detail_p">Ligation of gene_<i>leudh</i> and terminator</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of gene and terminator_B0015</br>
+. Double enzyme digestion of gene_<i>leudh</i> and terminator_B0015</br>
-. Electrophoresis analysis of double digested result of plasmid</br>
+. Electrophoresis analysis of double digested result of plasmid.</br>
-. Extract double digested gene</br>
+. Extract double digested gene_<i>leudh</i>.</br>
-. Cycle purity of digested terminator</br>
+. Cycle purity of digested terminator.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/3/34/Amoy-Notebook_node35-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/3/34/Amoy-Notebook_node35-1.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">plasmid of gene ldh and terminator</br></p>
+<p class="detail_p">Plasmid of gene_<i>leudh</i> and terminator_B0015</br></p>
 </div>
 </div>
@@ Line 437: / Line 440: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of gene and terminator</br></p>
+<p class="detail_p">Ligation of gene_<i>fdh</i> and terminator</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of gene and terminator_B0015</br>
+. Double enzyme digestion of gene_<i>fdh</i> and terminator_B0015</br>
-. Electrophoresis analysis of double digested result of plasmid</br>
+. Electrophoresis analysis of double digested result of plasmid.</br>
-. Extract double digested gene</br>
+. Extract double digested gene_<i>fdh</i>.</br>
-. Cycle purity of digested terminator</br>
+. Cycle purity of digested terminator.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/01/Amoy-Notebook_Node36_figure1.JPG" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">plasmid of gene fdh and terminator</br></p>
+<p class="detail_p">Plasmid of gene_<i>fdh</i> and terminator_B0015</br></p>
 </div>
 </div>
@@ Line 461: / Line 464: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of gene and terminator</br></p>
+<p class="detail_p">Ligation of gene_<i>leudh</i> and terminator</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of gene and terminator_B1006</br>
+. Double enzyme digestion of gene_<i>leudh</i> and terminator_B1006</br>
-. Electrophoresis analysis of double digested result of plasmid</br>
+. Electrophoresis analysis of double digested result of plasmid.</br>
-. Extract double digested gene</br>
+. Extract double digested gene_<i>leudh</i> and terminator.</br>
-. Cycle purity of digested terminator</br>
+. Ligate under 16℃ for 8 hours.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Transformation</br></p>
-. Transformation</br></p>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c1/Amoy-Notebook_node37-1.jpeg" />
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c1/Amoy-Notebook_node37-1.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">plasmid of gene ldh and terminator</br></p>
+<p class="detail_p">Plasmid of gene_<i>leudh</i> and terminator_B1006</br></p>
 </div>
 </div>
@@ Line 485: / Line 487: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of gene and terminator</br></p>
+<p class="detail_p">Ligation of gene_<i>fdh</i> and terminator</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of gene and terminator_B1006</br>
+. Double enzyme digestion of gene_<i>fdh</i> and terminator_B1006</br>
-. Electrophoresis analysis of double digested result of plasmid</br>
+. Electrophoresis analysis of double digested result of plasmid.</br>
-. Extract double digested gene</br>
+. Extract double digested gene_<i>fdh</i> and terminator.</br>
-. Cycle purity of digested terminator</br>
+. Ligate under 16℃ for 8 hours.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Transformation</br></p>
-. Transformation</br></p>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node38-1.jpeg" />
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node38-1.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">plasmid of gene and terminator</br></p>
+<p class="detail_p">Plasmid of gene_<i>fdh</i> and terminator_B1006</br></p>
 </div>
 </div>
@@ Line 509: / Line 510: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Ligation of isolated circuit with RBS_B0032 and gene_<i>leudh</i></br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of LacI_B0032 and LeuDH_T</br>
+. Double enzyme digestion of Plac_B0032 and LeuDH_T.</br>
-. Electrophoresis analysis of double digested result</br></p>
+. Electrophoresis analysis of double digested result.</br>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/a/aa/Amoy-Notebook_node21-1.jpeg" />
+. Extract double digested products.</br>
+. Ligate under 16℃ for 8 hours.</br>
+. Transformation</br>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/57/Amoy-Notebook_node21-2.JPG" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Extract the plasmids.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Electrophoresis analysis of plasmids.</br></p>
-. Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c4/Amoy-Notebook_node21-2.jpeg" />
-<p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
-. Extract the plasmids</br>
-. Electrophoresis analysis of plasmids</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Isolated circuit with RBS_B0032 and gene_<i>leudh</i></br></p>
 </div>
 </div>
@@ Line 536: / Line 533: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Ligation of isolated circuit with RBS_B0034 and gene_<i>leudh</i></br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of LacI_B0032 and LeuDH_T</br>
+. Double enzyme digestion of Plac_B0034 and LeuDH_TT</br>
-. Electrophoresis analysis of double digested result</br></p>
+. Electrophoresis analysis of double digested result.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1b/Amoy-Notebook_node22-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e2/Amoy-Notebook_Node2_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Extract double digested products.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Transformation</br></p>
-. Transformation</br></p>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/43/Amoy-Notebook_node24-2.JPG" />
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/70/Amoy-Notebook_node22-2.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
 . Extract the plasmids</br>
 . Electrophoresis analysis of plasmids</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f9/Amoy-Notebook_node22-3.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e3/Amoy-Notebook_Node22_figure3.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Isolated circuit with RBS_B0034 and gene_<i>leudh</i></br></p>
 </div>
 </div>
@@ Line 563: / Line 559: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Ligation of isolated circuit with RBS_B0034 and gene_<i>fdh</i></br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of LacI_B0032 and LeuDH_T</br>
+. Double enzyme digestion of Plac_B0032 and LeuDH_T</br>
 . Electrophoresis analysis of double digested result</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/45/Amoy-Notebook_node23-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e2/Amoy-Notebook_Node2_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Extract double digested products.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+. Transformation</br></p>
-. Transformation</br></p>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/3/3e/Amoy-Notebook_node23-2.JPG" />
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/0e/Amoy-Notebook_node23-2.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f7/Amoy-Notebook_node23-3.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/d/d7/Amoy-Notebook_Node23_figure3.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Isolated circuit with RBS_B0034 and gene_<i>fdh</i></br></p>
 </div>
 </div>
@@ Line 590: / Line 585: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">make connection of isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Ligation of isolated circuit with RBS_B0030 and gene_<i>leudh</i></br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of LacI_B0032 and LeuDH_T</br>
+. Double enzyme digestion of P<sub>J23100</sub>_B0030 and LeuDH_T</br>
-. Electrophoresis analysis of double digested result</br></p>
+. Electrophoresis analysis of double digested result.</br>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+. Extract double digested products.</br>
-<p class="detail_p"></br>
+. Ligate under 16℃ for 8 hours.</br>
-. Extract double digested product</br>
+. Transformation</br>
-. Link gene with terminator under 16℃ for 8 hours</br>
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f8/Amoy-Notebook_Node24_figure2.JPG" />
-. Link gene with terminator under 16℃ for 8 hours</br>
-. Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/e7/Amoy-Notebook_node24-2.jpeg" />
 <p class="detail_p"></br>
-. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c9/Amoy-Notebook_Node24_figure3.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">isolated circuit with RBS_B0032 and gene_ldh</br></p>
+<p class="detail_p">Isolated circuit with RBS_B0030 and gene_<i>leudh</i></br></p>
 </div>
 </div>
@@ Line 622: / Line 614: @@
 . Double enzyme digestion of P<sub>lac</sub> and RBS_B0032</br>
 . Electrophoresis analysis of double digested result of plasmid</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_Node32_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/50/Amoy-Notebook_Node42_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested promoter LacI</br>
+. Extract double digested Plac</br>
-. Cycle purity of digested rbs_B0032</br>
+. Cycle purity of digested RBS_B0032</br>
-. Link promoter with rbs under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
-. transformation</br></p>
+. Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/7a/Amoy-Notebook_node32-2.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/7a/Amoy-Notebook_node32-2.jpeg" />
 <p class="detail_p"></br>
-. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br>
+. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c9/Amoy-Notebook_Node32_figure3.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/fa/Amoy-Notebook_Node42_figure3.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> Plasmid of LacI linked with RBS_B0032</br></p>
+<p class="detail_p"> Plasmid of Plac linked with RBS_B0032</br></p>
 </div>
 </div>
@@ Line 647: / Line 639: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of circuits with RBS_B0032_gene_<i>ldh</i> and RBS_B0034_gene_<i>fdh</i>. </br>
+. Double enzyme digestion of circuits with RBS_B0032_gene_<i>leudh</i> and RBS_B0034_gene_<i>fdh</i>. </br>
 . Electrophoresis analysis of double digested result.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_Node32_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/2/2c/Amoy-Notebook_Node11_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Extract double digested products.</br>
-. Ligate under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/e/ec/Amoy-Notebook_node11-2.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/b/b9/Amoy-Notebook_node11-2.JPG" />
 <p class="detail_p"></br>
 . Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br>
+. Electrophoresis analysis of plasmids.</br>
-. Verify the results by double enzyme digestion</br></p>
+. Verify the results by double enzyme digestion.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_node11-3.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/80/Amoy-Notebook_Node11_figure3.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">final circuit of RBS_B0032</br></br></br></p>
+<p class="detail_p">Final circuit of RBS_B0032</br></br></br></p>
 </div>
 </div>
@@ Line 674: / Line 666: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of circuit with RBS_B0034_gene_<i>ldh</i> and RBS_B0034_gene_<i>fdh</i>.</br>
+. Double enzyme digestion of circuit with RBS_B0034_gene_<i>leudh</i> and RBS_B0034_gene_<i>fdh</i>.</br>
-. Electrophoresis analysis of double digested result</br></p>
+. Electrophoresis analysis of double digested result.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_Node32_figure1.jpg" />
+<img style="width: 60%; margin-right:40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/5/51/Amoy-Notebook_Node12_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Extract double digested products.</br>
-. Ligate under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/01/Amoy-Notebook_node12-2.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/0/01/Amoy-Notebook_node12-2.jpeg" />
 <p class="detail_p"></br>
 . Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/7/7a/Amoy-Notebook_node12-3.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/4/4e/Amoy-Notebook_Node12_figure3.png" />
 <p class="detail_p"></br>
-. Verify the results by double enzyme digestion</br></p>
+. Verify the results by double enzyme digestion.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/2/2d/Amoy-Notebook_node12-4.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/9/9f/Amoy-Notebook_Node12_figure4.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">final circuit of RBS_B0034</br></br></br></p>
+<p class="detail_p">Final circuit of RBS_B0034</br></br></br></p>
 </div>
 </div>
@@ Line 703: / Line 695: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of circuit with RBS_B0030_gene_<i>ldh</i> and RBS_B0034_gene_<i>fdh</i>.</br>
+. Double enzyme digestion of circuit with RBS_B0030_gene_<i>leudh</i> and RBS_B0034_gene_<i>fdh</i>.</br>
 . Electrophoresis analysis of double digested result</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_Node32_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/a/ae/Amoy-Notebook_Node13_figure1.png" />
 <p class="detail_p"></br>
-. Extract double digested product</br>
+. Extract double digested products.</br>
-. Ligate under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1f/Amoy-Notebook_node13-2.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node13-2.JPG" />
 <p class="detail_p"></br>
 . Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/f/f3/Amoy-Notebook_node13-3.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/2/29/Amoy-Notebook_Node13_figure3.png" />
 <p class="detail_p"></br>
-. Verify the results by double enzyme digestion</br></p>
+. Verify the results by double enzyme digestion.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c5/Amoy-Notebook_node13-4.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/c7/Amoy-Notebook_Node13_figure4.png" />
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">final circuit of RBS_B0030</br></br></br></p>
+<p class="detail_p">Final circuit of RBS_B0030</br></br></br></p>
 </div>
 </div>
@@ Line 732: / Line 724: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Add 20ul ddH20 to solve the dry powder</br>
+. Add 20μL ddH<sub>2</sub>O to solve the dry powder.</br>
-. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p>
+. Suck 10μL of plasmid into 50μL of competent cell for transformation.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/c/cf/Amoy-Notebook_node33-1.JPG" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of chloramphenicol for 12h</br>
+. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br>
-. Plasmid minipre</br></p>
+. Plasmid Extraction</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> </br></p>
+<p class="detail_p"> Plasmid of Plac_RBS_B0034</br></p>
 </div>
 </div>
@@ Line 752: / Line 744: @@
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Add 20ul ddH20 to solve the dry powde</br>
+. Add 20μL ddH<sub>2</sub>O to solve the dry powder.</br>
-. Suck 10ul of plasmid into 50ul of competent cell for transformation</br></p>
+. Suck 10μL of plasmid into 50μL of competent cell for transformation.</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/8/87/Amoy-Notebook_Node41_figure1.jpg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/1a/Amoy-Notebook_node34-1.JPG" />
 <p class="detail_p"></br>
 . Pick a single colony from the agar plate using a sterile pipette tip. </br>
-. Culture at 10ml LB of chloramphenicol for 12h</br>
+. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.</br>
-. Plasmid minipre</br></p>
+. Plasmid Extraction</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p"> </br></p>
+<p class="detail_p"> Plasmid of P<sub>J23100</sub>_RBS_B0030</br></p>
 </div>
 </div>
@@ Line 769: / Line 761: @@
 <div style="width: 80%; margin-left: 10%;">
 <p class="detail_h1">Purpose:</br></p>
-<p class="detail_p">Make connection of promoter and rbs</br></p>
+<p class="detail_p">Ligation of promoter and RBS</br></p>
 <p class="detail_h1">Steps:</br></p>
 <p class="detail_p">
-. Double enzyme digestion of promoter_J23100 and RBS_B0034</br>
+. Double enzyme digestion of P<sub>J23100</sub> and RBS_B0034.</br>
-. Cycle purity of digested products</br>
+. Cycle purity of digested products.</br>
-. Link promoter with rbs under 16℃ for 8 hours</br>
+. Ligate under 16℃ for 8 hours.</br>
 . Transformation</br></p>
-<img style="width: 30%; margin-right: 70%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node31-1.jpeg" />
+<img style="width: 60%; margin-right: 40%; margin-top: 10px; margin-bottom: 0px;" src="https://static.igem.org/mediawiki/2015/1/18/Amoy-Notebook_node31-1.jpeg" />
 <p class="detail_p"></br>
-. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of amp</br>
+. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.</br>
-. Extract the plasmids</br>
+. Extract the plasmids.</br>
-. Electrophoresis analysis of plasmids</br></p>
+. Electrophoresis analysis of plasmids.</br></p>
 <p class="detail_h1">Product:</br></p>
-<p class="detail_p">Plasmid of promoter J23100 linked with RBS_B0034</br></p>
+<p class="detail_p">Plasmid of P<sub>J23100</sub> linked with RBS_B0034</br></p>
 </div>
 </div>
 <span id="node31_close" style="background: #f0f0f0 url(https://static.igem.org/mediawiki/2015/7/73/GalleryClose.gif) no-repeat center center; position: fixed; height: 18px; width: 18px; cursor: pointer; margin-top: 60px; right: 12%; z-index: 1002; display: none;"></span>
@@ Line 802: / Line 793: @@
 <!--top_menu-->
-<div id='cssmenu'>
+<span class="preload1"></span> <span class="preload2"></span>
-<ul>
+<ul id="nav">
-   <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Team'>Team</a>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Team" id="products" class="top_link"><span class="down">TEAM</span></a>
-      <ul>
+    <ul class="sub">
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Team#member_student'>Member</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Team#member_student">Member</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Member/Amoy'>Amoy</a></li>
+       <li><a href="https://2015.igem.org/Team:Amoy/Member/Amoy">Amoy</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Attributions'>Attributions</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Attributions">Attributions</a></li>
-      </ul>
+    </ul>
-   </li>
+  </li>
-   <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Project'>Project</a>
-      <ul>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Project/Background'>Background</a></li>
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-       </ul>
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-      <ul>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Notebook/Notebook'>Notebook</a></li>
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-   <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Newsletter'>Newsletter</a>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Project" id="products" class="top_link"><span class="down">PROJECT</span></a>
-       <ul>
+    <ul class="sub">
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Newsletter#title'>Introduction</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Project/Background">Background</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Newsletter/Contribution'>Contribution</a></li>
+       <li><a href="https://2015.igem.org/Team:Amoy/Description">Description</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Newsletter/Discussion'>Discussion</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Project/Methods">Methods</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Newsletter/Links'>Links</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Project/Results">Results</a></li>
-      </ul>
+      <li><a href="https://2015.igem.org/Team:Amoy/Project/Discussion">Discussion</a></li>
-   </li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Project/FutureWork">Future Work</a></li>
-   <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Practices'>Practices</a>
+    </ul>
-      <ul>
+  </li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Practices/Promotion'>Promotion</a></li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Practices/Talk'>Talk</a></li>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Notebook" id="products" class="top_link"><span class="down active">NOTEBOOK</span></a>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Practice/Communication'>Communication</a></li>
+    <ul class="sub">
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Collaborations'>Collaborations</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Notebook/Notebook">Notebook</a></li>
-      </ul>
+      <li><a href="https://2015.igem.org/Team:Amoy/Notebook/Protocol">Protocols</a></li>
-   </li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Parts">Parts</a></li>
-   <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Judging'>Judging</a>
+      <li><a href="https://2015.igem.org/Team:Amoy/Notebook/Gallery">Gallery</a></li>
-      <ul>
+    </ul>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Judging/Medal'>Medal Criteria</a></li>
+  </li>
-         <li class='has-sub'><a href='https://2015.igem.org/Team:Amoy/Judging/Acknowledgement'>Acknowledgement</a></li>
-      </ul>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Interlab" id="products" class="top_link"><span class="down">INTERLAB</span></a></li>
-   </li>
-   <li><a href='https://2015.igem.org/Team:Amoy/Safety'>Safety</a></li>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Newsletter" id="products" class="top_link"><span class="down">NEWSLETTER</span></a>
+    <ul class="sub">
+      <li><a href="https://2015.igem.org/Team:Amoy/Newsletter#title">Introduction</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Newsletter/Contribution">Contribution</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Newsletter/Discussion">Discussion</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Newsletter/Links">Links</a></li>
+    </ul>
+  </li>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Practices" id="products" class="top_link"><span class="down">PRACTICES</span></a>
+    <ul class="sub">
+      <li><a href="https://2015.igem.org/Team:Amoy/Practices/Promotion">Promotion</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Practices/Talk">Talk</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Practice/Communication">Communication</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Collaborations">Collaborations</a></li>
+    </ul>
+  </li>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Judging" id="products" class="top_link"><span class="down">JUDGING</span></a>
+    <ul class="sub">
+      <li><a href="https://2015.igem.org/Team:Amoy/Judging/Medal">Medal Criteria</a></li>
+      <li><a href="https://2015.igem.org/Team:Amoy/Judging/Acknowledgement">Acknowledgement</a></li>
+    </ul>
+  </li>
+  <li class="top"><a href="https://2015.igem.org/Team:Amoy/Safety" id="products" class="top_link"><span class="down">SAFETY</span></a></li>
 </ul>
-</div>
 </div>
@@ Line 878: / Line 874: @@
 <div id="title" style="width: 70%; margin-left: 25%;">
 <p id="title_p">NOTEBOOK</p>
-<p class="main_p">Initially, they used isolated enzymes, which can be disadvantageous for the reason that enzymes are  always destabilized in the isolation and purification process. What's more, the cofactor-NADH is rather an expensive raw material, which will enhance the cost of L-tert-leucine production. So scientists introduced whole-cell biocatalysts to L-tert-leucine production. Whole-cell biocatalysts could stabilize enzymes and reduce the addition level of cofactor NADH.</br></br>
+<p class="main_p">Initially, they used isolated enzymes, which can be disadvantageous for the reason that enzymes are  always destabilized in the isolation and purification process. What's more, the cofactor NADH is rather an expensive raw material, which will enhance the cost of L-<i>tert</i>-leucine production. So scientists introduced whole-cell biocatalysts to L-<i>tert</i>-leucine production. Whole-cell biocatalysts could stabilize enzymes and reduce the addition level of cofactor NADH.</br></br>
-In the path of building our biobricks, we divided the circuits into two modules. One is promoter linked with rbs and the other is gene linked with terminator. The dendrogram below is our experiments detail. Click each bottom for more information.</br></br>
+In the path of building our biobricks, we divided the circuits into two modules. One is promoter linked with RBS and the other is gene linked with terminator. The dendrogram below is our experiments detail. Click each bottom for more information.</br></br>
 </p>
@@ Line 918: / Line 914: @@
 </svg>
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+<a id="node11" class="btn btn-success" rel="popover" style="border-radius: 100px; width: 30px; height: 30px; position: absolute; margin-left: 285px; margin-top: 35px; background-color: green; border: 0px;" data-trigger="hover" data-content="Plac_B0032_LeuDH_T_LacI_B0034_FDH_TT" ></a>
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+<a id="node12" class="btn btn-success" rel="popover" style="border-radius: 100px; width: 30px; height: 30px; position: absolute; margin-left: 385px; margin-top: 35px; background-color: green; border: 0px;" data-trigger="hover" data-content="Plac_B0034_LeuDH_TT_LacI_B0034_FDH_TT" ></a>
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+<a id="node13" class="btn btn-success" rel="popover" style="border-radius: 100px; width: 30px; height: 30px; position: absolute; margin-left: 485px; margin-top: 35px; background-color: green; border: 0px;" data-trigger="hover" data-content="P<sub>J23100</sub>_B0030_LeuDH_T_LacI_B0034_FDH_TT" ></a>
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+<a id="node21" class="btn btn-success" rel="popover" style="border-radius: 100px; width: 30px; height: 30px; position: absolute; margin-left: 235px; margin-top: 135px; background-color: yellow; border: 0px;" data-trigger="hover" data-content="Plac_B0032_leuDH_T" ></a>
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@@ Line 936: / Line 932: @@
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Latest revision as of 03:14, 19 September 2015

Aomy/Project

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powder.
2. Suck 10μl of plasmid into 50μl of competent cell for transformation.

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.
5. Plasmid extraction.

Product:

Plasmid of promoter_J23100

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powder
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm.
5. Plasmid extraction.

Product:

Plasmid of promoter_LacI

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powder
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm
5. Plasmid Extraction

Product:

Plasmid of RBS_B0034

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powder
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of ampicillin for 12h, 37℃, 200rpm
5. Plasmid Extraction

Product:

Plasmid of RBS_B0032

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powder
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm
5. Plasmid Extraction

Product:

Plasmid of RBS_B0030

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μL ddH₂O to solve the dry powder.
2. Suck 10μL of plasmid into 50μL of competent cell for transformation.

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.
5. Plasmid Extraction

Product:

Plasmid of Plac_RBS_B0034

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μL ddH₂O to solve the dry powder.
2. Suck 10μL of plasmid into 50μL of competent cell for transformation.

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.
5. Plasmid Extraction

Product:

Plasmid of P_J23100_RBS_B0030

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powde
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm
5. Plasmid Extraction

Product:

Plasmid of terminator_B0015

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μl ddH₂O to solve the dry powde
2. Suck 10μl of plasmid into 50μl of competent cell for transformation

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm
5. Plasmid Extraction

Product:

Plasmid of terminator_B1006

Purpose:

PCR amplification for gene_leudh and double enzyme digestion

Steps:

1. PCR amplification system for gene_leudh

Components	Volume
ddH₂O	16μL
leudh-F	1.5μL
leudh-R	1.5μL
pUB18-leudh	1μL
Prime Star	20μL

2. Electrophoresis of PCR products of gene_leudh
3. Double enzyme digestion of gene_leudh

Components	Volume
Gene	20μL
ddH_{2_O}	20μL
buffer	10μL
EcoR I	5μL
Spe I	5μL

4. Cycle purity of digested gene_leudh

Product:

Digested gene_leudh

Purpose:

PCR amplification for gene_fdh and double enzyme digestion

Steps:

1. PCR amplification system for gene_fdh

Components	Volume
ddH₂O	16μL
fdh-F	1.5μL
fdh-R	1.5μL
pUB18-fdh	1μL
Prime Star	20μL

2. Electrophoresis of PCR products of gene_fdh
3. Double enzyme digestion of gene_fdh

Components	Volume
Gene	50μL
ddH₂O	10μL
buffer	10μL
EcoR I	5μL
Spe I	5μL

4. Cycle purity of digested gene_fdh

Product:

Digested gene_fdh

Purpose:

Ligation of gene_leudh and terminator

Steps:

1. Double enzyme digestion of gene_leudh and terminator_B0015
2. Electrophoresis analysis of double digested result of plasmid.
3. Extract double digested gene_leudh.
4. Cycle purity of digested terminator.
5. Ligate under 16℃ for 8 hours.
6. Transformation

7. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.
8. Extract the plasmids.
9. Electrophoresis analysis of plasmids.

Product:

Plasmid of gene_leudh and terminator_B0015

Purpose:

Ligation of gene_fdh and terminator

Steps:

1. Double enzyme digestion of gene_fdh and terminator_B0015
2. Electrophoresis analysis of double digested result of plasmid.
3. Extract double digested gene_fdh.
4. Cycle purity of digested terminator.
5. Ligate under 16℃ for 8 hours.
6. Transformation

Product:

Plasmid of gene_fdh and terminator_B0015

Purpose:

Ligation of gene_leudh and terminator

Steps:

1. Double enzyme digestion of gene_leudh and terminator_B1006
2. Electrophoresis analysis of double digested result of plasmid.
3. Extract double digested gene_leudh and terminator.
4. Ligate under 16℃ for 8 hours.
5. Transformation

6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.
7. Extract the plasmids.
8. Electrophoresis analysis of plasmids.

Product:

Plasmid of gene_leudh and terminator_B1006

Purpose:

Ligation of gene_fdh and terminator

Steps:

1. Double enzyme digestion of gene_fdh and terminator_B1006
2. Electrophoresis analysis of double digested result of plasmid.
3. Extract double digested gene_fdh and terminator.
4. Ligate under 16℃ for 8 hours.
5. Transformation

Product:

Plasmid of gene_fdh and terminator_B1006

Purpose:

Ligation of isolated circuit with RBS_B0032 and gene_leudh

Steps:

1. Double enzyme digestion of Plac_B0032 and LeuDH_T.
2. Electrophoresis analysis of double digested result.
3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

Product:

Isolated circuit with RBS_B0032 and gene_leudh

Purpose:

Ligation of isolated circuit with RBS_B0034 and gene_leudh

Steps:

1. Double enzyme digestion of Plac_B0034 and LeuDH_TT
2. Electrophoresis analysis of double digested result.

3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

6. Pick 8 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.
7. Extract the plasmids
8. Electrophoresis analysis of plasmids

Product:

Isolated circuit with RBS_B0034 and gene_leudh

Purpose:

Ligation of isolated circuit with RBS_B0034 and gene_fdh

Steps:

1. Double enzyme digestion of Plac_B0032 and LeuDH_T
2. Electrophoresis analysis of double digested result

3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

Product:

Isolated circuit with RBS_B0034 and gene_fdh

Purpose:

Ligation of isolated circuit with RBS_B0030 and gene_leudh

Steps:

1. Double enzyme digestion of P_J23100_B0030 and LeuDH_T
2. Electrophoresis analysis of double digested result.
3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

Product:

Isolated circuit with RBS_B0030 and gene_leudh

Purpose:

Ligation of promoter and RBS_B0032

Steps:

1. Double enzyme digestion of P_lac and RBS_B0032
2. Electrophoresis analysis of double digested result of plasmid

3. Extract double digested Plac
4. Cycle purity of digested RBS_B0032
5. Ligate under 16℃ for 8 hours.
6. Transformation

Product:

Plasmid of Plac linked with RBS_B0032

Purpose:

Ligation of the final circuit with RBS_B0032

Steps:

1. Double enzyme digestion of circuits with RBS_B0032_gene_leudh and RBS_B0034_gene_fdh.
2. Electrophoresis analysis of double digested result.

3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

Product:

Final circuit of RBS_B0032

Purpose:

Ligation of the final circuit with RBS_B0034

Steps:

1. Double enzyme digestion of circuit with RBS_B0034_gene_leudh and RBS_B0034_gene_fdh.
2. Electrophoresis analysis of double digested result.

3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

9. Verify the results by double enzyme digestion.

Product:

Final circuit of RBS_B0034

Purpose:

Ligation of the final circuit with RBS_B0030

Steps:

1. Double enzyme digestion of circuit with RBS_B0030_gene_leudh and RBS_B0034_gene_fdh.
2. Electrophoresis analysis of double digested result

3. Extract double digested products.
4. Ligate under 16℃ for 8 hours.
5. Transformation

9. Verify the results by double enzyme digestion.

Product:

Final circuit of RBS_B0030

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μL ddH₂O to solve the dry powder.
2. Suck 10μL of plasmid into 50μL of competent cell for transformation.

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.
5. Plasmid Extraction

Product:

Plasmid of Plac_RBS_B0034

Purpose:

Extract plasmid from dry powder

Steps:

1. Add 20μL ddH₂O to solve the dry powder.
2. Suck 10μL of plasmid into 50μL of competent cell for transformation.

3. Pick a single colony from the agar plate using a sterile pipette tip.
4. Culture at 10ml LB of chloramphenicol for 12h, 37℃, 200rpm.
5. Plasmid Extraction

Product:

Plasmid of P_J23100_RBS_B0030

Purpose:

Ligation of promoter and RBS

Steps:

1. Double enzyme digestion of P_J23100 and RBS_B0034.
2. Cycle purity of digested products.
3. Ligate under 16℃ for 8 hours.
4. Transformation

5. Pick 10 single colonies from the agar plate using sterile pipette tips. Put it into 10ml LB of chloramphenicol. Culture at 37℃,200rpm for 12~14 hours.
6. Extract the plasmids.
7. Electrophoresis analysis of plasmids.

Product:

Plasmid of P_J23100 linked with RBS_B0034

TEAM
- Member
- Amoy
- Attributions
PROJECT
- Background
- Description
- Methods
- Results
- Discussion
- Future Work
NOTEBOOK
- Notebook
- Protocols
- Parts
- Gallery
INTERLAB
NEWSLETTER
PRACTICES
JUDGING
- Medal Criteria
- Acknowledgement
SAFETY

Notebook

Notebook
Protocols
Parts
Gallery

NOTEBOOK

Initially, they used isolated enzymes, which can be disadvantageous for the reason that enzymes are always destabilized in the isolation and purification process. What's more, the cofactor NADH is rather an expensive raw material, which will enhance the cost of L-tert-leucine production. So scientists introduced whole-cell biocatalysts to L-tert-leucine production. Whole-cell biocatalysts could stabilize enzymes and reduce the addition level of cofactor NADH.

In the path of building our biobricks, we divided the circuits into two modules. One is promoter linked with RBS and the other is gene linked with terminator. The dendrogram below is our experiments detail. Click each bottom for more information.

Email: igemxmu@gmail.com

Website: 2015.igem.org/Team:Amoy

Address: Xiamen University, No. 422, Siming South Road, Xiamen, Fujian, P.R.China 361005