Difference between revisions of "Team:Tianjin/Note/6803"

 
(63 intermediate revisions by 5 users not shown)
Line 1: Line 1:
 
{{:Team:Tianjin/Templates/MaterialTheme|}}
 
{{:Team:Tianjin/Templates/MaterialTheme|}}
  
{{:Team:Tianjin/Templates/AddCSS|:Team:Tianjin/Note/6803/camarts.css}}
+
{{:Team:Tianjin/Templates/AddCSS|:Team:Tianjin/Note/R-R/camarts.css}}
 
{{:Team:Tianjin/Templates/AddCSS|:Team:Tianjin/Experiment/css/font.css}}
 
{{:Team:Tianjin/Templates/AddCSS|:Team:Tianjin/Experiment/css/font.css}}
 
 
<html lang="en">
 
<html lang="en">
 +
<style>
 +
#Notes{
 +
  color: inherit;
 +
  background-color: rgba(255, 255, 255, 0.1);
 +
}
 +
</style>
 +
 
<head>
 
<head>
 
<meta charset="utf-8" />  
 
<meta charset="utf-8" />  
Line 12: Line 18:
  
 
<meta content="width=device-width, initial-scale=1.0, maximum-scale=1.0, user-scalable=0" name="viewport" />
 
<meta content="width=device-width, initial-scale=1.0, maximum-scale=1.0, user-scalable=0" name="viewport" />
 +
 +
 +
 +
<style>
 +
#Notes{
 +
  color: inherit;
 +
  background-color: rgba(255, 255, 255, 0.1);
 +
}
 +
</style>
  
 
<!------------------------------------------- This part should be dismissed in WIKI u
 
<!------------------------------------------- This part should be dismissed in WIKI u
Line 43: Line 58:
 
              
 
              
 
   <div id="Topp"></div>
 
   <div id="Topp"></div>
 
 
 
<div id="page" class="hfeed" >
 
<div id="page" class="hfeed" >
 
      
 
      
 
<div id="page-heading" class="relative">
 
<div id="page-heading" class="relative">
      <img class="ribbon-version1" src="images/ribbon-2016 - 副本.png">
+
   
 
      
 
      
 
     <header id="main-header" role="banner">
 
     <header id="main-header" role="banner">
      
+
     <style>
 +
.note-content,.note-content2,.note-content3,.note-content4,.note-content5,.note-content6,.note-content7,.note-content8,.note-content9,.note-content10,.note-content li,.note-content2 li,.note-content3 li,.note-content4 li,.note-content5 li,.note-content6 li,.note-content7 li,.note-content8 li,.note-content9 li,.note-content10 li{
 +
font-family:Arial;
 +
font-size:18px;
 +
text-align:justify;
 +
}
 +
</style>
 +
     
 
    
 
    
        <nav id="nav" class="nav" role="navigation"> 
+
     
            <a href="#nav" title="显示菜单" data-ajax="false">菜单</a>
+
            <a href="#" title="隐藏菜单" data-ajax="false">关闭</a>
+
            <ul role="menubar"> 
+
             
+
            </ul> 
+
        </nav>
+
 
     </div>
 
     </div>
 
</header>
 
</header>
   
+
 
 
<div id="main">         
 
<div id="main">         
 
       <div id="content" class="home blog single-author one-column content" role="main">
 
       <div id="content" class="home blog single-author one-column content" role="main">
     
 
  
<div id="Week1"></div>         
+
<div id="Week1"></div>         
 
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<header class="entry-header">
 
<header class="entry-header">
<div class="entry-title" align="center" >Notes</div>
+
<div class="entry-title" align="center" >Notes For Cyanobacteria</div>
 
</header><!-- .entry-header -->
 
</header><!-- .entry-header -->
        <h1 class="entry-title">Week1(8/1/2016-8/7/2016)</h1>
+
 
 +
 
 +
 
 +
<!------------------------------------week 1 start------------------------------------------------>
 +
<div id="Week1"></div>
 +
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<header class="entry-header">
 +
<h1 class="entry-title">Week1(7/31/2016-8/6/2016)</h1>
 +
</header><!-- .entry-header -->
 +
 
 
<div class="entry-content">
 
<div class="entry-content">
 +
<div class="note-content2">
  
  
<p>
 
    <li>Cultivation: 30µL mother liquid of Synechococcus sp. PCC 7942 (wild type)were cultivated in 10 mL BG-11-media at 30°C and 140rpm.<br/></li>
 
<li>The genome DNA of 7942 was extracted using a Genomic DNA Isolation Kit.</li>
 
                        </p>
 
         
 
         
 
       
 
<hr class="article">
 
    </article><!-- #post-4252 -->
 
  
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Jul.31th</b></h1>
 +
<div style="padding-left:32px;"><li>Cultivation: 30µL mother liquid of Synechococcus sp PCC 7942 (wild type)were cultivated in 10 mL BG-11-media at 30°C and 140rpm.</li>
  
  
 +
<li>The genome DNA of 7942 was extracted using a Genomic DNA Isolation Kit.</li></div><br/>
  
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<header class="entry-header">
 
<h1 class="entry-title">Week2(8/15/2016-8/21/2016)</h1>
 
</header><!-- .entry-header -->
 
  
<div class="entry-content">
+
</div>
<p><li>Synechococcus sp PCC 7942 had no signals of life.</li><br />
+
<div id="Week2"></div>
 +
<a class="expand-btn2">Show More</a>
  
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/2016/3/37/Igem--6803-week2.jpg"  alt="IMG_2956" width="800" height="533"
+
 
</a>
+
 
 +
</div><!-- .entry-content -->
 +
 
 +
 
          
 
          
<hr class="article">
 
 
    </article>
 
    </article>
  
 
          
 
          
  
 +
<!------------------------------------week1 end------------------------------------------------>
 +
  
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
+
   
<h1 class="entry-title">Week3(8/29/2016-9/4/2016)</h1>
+
         
 +
 
 +
 
 +
 
 +
<!------------------------------------week2 start------------------------------------------------>     
 +
 
 +
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<h1 class="entry-title">Week2(8/14/2016-8/20/2016)</h1>
 
<div class="entry-content">
 
<div class="entry-content">
<p><li>pMV-G19</li>
 
<li>pMV-G15</li>
 
<li>Colonies were used to inoculate overnight cultures.</li>
 
<li>Plasmids were isolated using a miniprep kit.</li>
 
  
<b>Amplification of <i>19</i> and <i>15</i> with Q5 High-Fidelity DNA Polymerase out of E.coli </b><br/>
 
  
 +
<div class="note-content4">
  
<div class="note-content">
 
  
  
  
<li><i>19</i> amplification at 65.0°C with 19.rev/fwd primes.</li>
 
  PCR worked, positive control worked, no amplification of <i>19</i>.
 
<li><i>15</i> amplification at 65.0°C with 15.rev/fwd primes.</li>
 
  PCR worked, positive control worked, no amplification of <i>15</i>.
 
<li>A product length of 900 bp was expected. The gel shows that most plasmids seem to be correct.</li>
 
<li>This result was confirmed by sequencing.</li>
 
<li>The fragments of <i>19</i> and <i>15</i> were purified with PCR Purification Kit.</li>
 
  
         
+
 
       
+
<div style="padding-left:32px;"><li>Synechococcus sp PCC 7942 had no signals of life.</li></div><br/>
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
<a href="https://static.igem.org/mediawiki/2016/3/37/Igem--6803-week2.jpg" data-lightbox="no" data-title="7942">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/3/37/Igem--6803-week2.jpg"  alt="Igem-6803-week2" width="300px"><br/><br/>
 +
</a>
 +
<br/> 
  
 
  </div>
 
  </div>
<a class="expand-btn">Show More</a>
 
  
 +
<div id="Week3"></div>
 +
<a class="expand-btn4">Show More</a>
  
<b>Ligation of <i>15</i> with <i>19</i></b><br/>
 
  
<div class="note-content2">
 
  
 +
 +
 +
</div><!-- .entry-content -->
 +
 +
 +
       
 +
 +
    </article>
 +
 +
 +
<!------------------------------------week2 end------------------------------------------------>
 +
 +
 +
 +
 +
 +
 +
 +
 +
<!------------------------------------week3 start------------------------------------------------>       
 +
 +
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<header class="entry-header">
 +
<h1 class="entry-title">Week3(8/28/2016-9/3/2016)</h1>
 +
</header><!-- .entry-header -->
 +
 +
<div class="entry-content">
 +
<div class="note-content4">
 +
 +
 +
 +
 +
 +
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Aug.29th</b></h1>
 +
<div style="padding-left:32px;"><li>pMV-G19 and pMV-G15  containing our target genes were received.</li><br/>
 +
 +
<a href="https://static.igem.org/mediawiki/2016/6/6d/Igem-6803-week3-1.jpg" data-lightbox="no" data-title="pMV-G19 and pMV-G15">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/6/6d/Igem-6803-week3-1.jpg"  alt="Igem-6803-week3-1" width="300px" ><br/><br/>
 +
</a>
 +
<br/>
 +
<li>Colonies were used to inoculate overnight cultures.</li>
 +
</div>
 +
<br/>
 +
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Aug.30th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids were isolated using a miniprep kit.</li>
 +
<li>Amplification of <i>19</i> and <i>15</i> with Q5 High-Fidelity DNA Polymerase out of E.coli.</li>
 +
&nbsp;&nbsp;<i>19</i> amplification at 65.0°C with 19.rev/fwd primes.<br/>
 +
&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;PCR worked, positive control worked, no amplification of <i>19</i>.<br/>
 +
&nbsp;&nbsp;<i>15</i> amplification at 65.0°C with 15.rev/fwd primes.<br/>
 +
&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;PCR worked, positive control worked, no amplification of <i>15</i>.<br/>
 +
<li>A product length of 900 bp was expected. The gel shows that most plasmids seem to be correct.</li>
 +
&nbsp;&nbsp;This result was confirmed by sequencing.<br/>
 +
<li>The fragments of <i>19</i> and <i>15</i> were purified with PCR Purification Kit.</li>
 +
</div>
 +
<br/>
 +
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Aug.31th</b></h1>
 +
<div style="padding-left:32px;"><li>Ligation of <i>15</i> with <i>19</i>.</li>
 
<li>We add a single 3`-adenine overhang to each end of the fragment of <i>19</i> and then purified with DNA Purification Kit.</li>
 
<li>We add a single 3`-adenine overhang to each end of the fragment of <i>19</i> and then purified with DNA Purification Kit.</li>
 
<li><i>19</i> was ligated into T vectors via TA clone and transformed into E.coli via heat shock.</li>
 
<li><i>19</i> was ligated into T vectors via TA clone and transformed into E.coli via heat shock.</li>
<li>A colony PCR was performed with five colonies.</li>
+
</div>
  Gel electrophoresis showed that 5 colonies were positive for insertion of <i>19</i>.</li>
+
<br/>
  Two of these colonies containing <i>19</i> were used to inoculate overnight cultures.</li>
+
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.1th</b></h1>
 +
<div style="padding-left:32px;"><li>A colony PCR was performed with five colonies.</li>
 +
<li>Gel electrophoresis showed that 5 colonies were positive for insertion of <i>19</i>.</li>
 +
<li>Two of these colonies containing <i>19</i> were used to inoculate overnight cultures.</li>
 
<li><i>15</i> gene fragment was phosphorylated.</li>
 
<li><i>15</i> gene fragment was phosphorylated.</li>
<li>Plasmids containing T vector with <i>19</i>(pT-19)were isolated using a miniprep kit.</li>
+
</div>
 +
<br/>
 +
 
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.2th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids containing T vector with <i>19</i>(pT-19)were isolated using a miniprep kit.</li>
 
<li>Mono-restriction digest of pT-19 with stu I. </li>
 
<li>Mono-restriction digest of pT-19 with stu I. </li>
 
<li>The enzyme-digested product was dephosphorylation.</li>
 
<li>The enzyme-digested product was dephosphorylation.</li>
 +
<br/>
 +
 +
<a href="https://static.igem.org/mediawiki/2016/a/aa/Igem-6803-week3.png" data-lightbox="no" data-title=" ">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/a/aa/Igem-6803-week3.png"  alt="Igem-6803-week3-2" width="800" height="533"><br/>
 +
</a>
 +
<br/>
 +
 
<li>Dephosphorylated plasmid and phosphorylated gene <i>15</i> were connected.</li>
 
<li>Dephosphorylated plasmid and phosphorylated gene <i>15</i> were connected.</li>
  Ligation product was transformed into E.coli via heat shock.</li>
+
<li>Ligation product was transformed into E.coli via heat shock.</li>
<li>A colony PCR was performed with twelve colonies.</li>
+
</div>
  Gel electrophoresis showed that 2 colonies were positive for connecting the plasmid and gene fragment.</li>
+
<br/>
  These two colonies were used to inoculate overnight cultures.</li>
+
<li>Plasmids with correct sequence of  <i>19-15</i>  were isolated using a miniprep kit.</li>
+
<li>Mono-restriction digest of pT-19-15 with Nru I.</li>
+
<li>The enzyme-digested product was dephosphorylation.</li>
+
  
         
+
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.3th</b></h1>
       
+
<div style="padding-left:32px;"><li>A colony PCR was performed with twelve colonies.</li>
 +
<li>Gel electrophoresis showed that 2 colonies were positive for connecting the plasmid and gene fragment.</li>
 +
<li>These two colonies were used to inoculate overnight cultures.</li>
 
</div>
 
</div>
            <a class="expand-btn2">Show More</a>
+
<br/>
  
  
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/igem.org/e/ec/T--Tianjin--cjw.jpg" alt="IMG_2956" width="800" height="533"  
+
 
</a>
+
</div>
 +
  <div id="Week4"></div>
 +
<a class="expand-btn4">Show More</a>
 +
 
 +
 
 +
</div><!-- .entry-content -->
 +
 
 +
 
          
 
          
<hr class="article">
 
 
    </article>
 
    </article>
  
 +
<!------------------------------------week3 end------------------------------------------------>
  
  
       
 
       
 
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<h1 class="entry-title">Week4(9/5/2016-9/11/2016)</h1>
 
<div class="entry-content">
 
<p><li>Colonies containing gene <i>13</i> were used to inoculate overnight cultures.</li>
 
<li>Plasmids were isolated using a miniprep kit.</li>
 
<b>Amplification of <i>13</i> with Q5 High-Fidelity DNA Polymerase out of E.coli </b><br/>
 
  
 +
<!------------------------------------week4 start------------------------------------------------>       
  
<div class="note-content3">
+
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<header class="entry-header">
 +
<h1 class="entry-title">Week4(9/4/2016-9/10/2016)</h1>
 +
</header><!-- .entry-header -->
  
 +
<div class="entry-content">
 +
<div class="note-content4">
 +
  
  
<li><i>13</i> amplification at 65.0°C with 13.rev/fwd primes</li>
 
PCR worked, positive control worked, no amplification of <i>13</i></li>
 
<li>The fragments of <i>13</i> were purified with PCR Purification Kit.</li>
 
<li><i>13</i> gene fragment was phosphorylated.</li>
 
         
 
       
 
  
</div>
 
<a class="expand-btn3">Show More</a>
 
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.4th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids with correct sequence of  <i>19-15</i>  were isolated using a miniprep kit.<li>
 +
<li>Mono-restriction digest of pT-19-15 with Nru I.</li>
 +
<li>The enzyme-digested product was dephosphorylation.</li>
 +
</div>
 +
<br/>
  
<b>Insertion of Ni promoter and ligation of <i>13-19-15</i></b><br/>
+
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.6th</b></h1>
 +
<div style="padding-left:32px;"><li>Colonies containing gene <i>13</i> were used to inoculate overnight cultures.
 +
</li>
 +
</div>
 +
<br/>
  
<div class="note-content4">
+
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.7th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids were isolated using a miniprep kit.</li>
 +
<li>Amplification of <i>13</i> with Q5 High-Fidelity DNA Polymerase out of E.coli </li>
 +
<li><i>13</i> amplification at 65.0°C with 13.rev/fwd primes</li>
 +
&nbsp;&nbsp;PCR worked, positive control worked, no amplification of <i>13</i><br/>
 +
<li>The fragments of <i>13</i> were purified with PCR Purification Kit.</li>
 +
</div>
 +
<br/>
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.8th</b></h1>
 +
<div style="padding-left:32px;"><li><i>13</i> gene fragment was phosphorylated.</li>
 +
</div>
 +
<br/>
  
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.9th</b></h1>
 +
<div style="padding-left:32px;"><li>Insertion of Ni promoter and ligation of <i>13-19-15</i></li>
 
<li>Ni inducible promoter was ligated into pCPC-3301 vector.</li>
 
<li>Ni inducible promoter was ligated into pCPC-3301 vector.</li>
 
<li>Phosphorylated <i>13</i> was ligated into pT-19-15 and transformed into E.coli via heat shock.</li>
 
<li>Phosphorylated <i>13</i> was ligated into pT-19-15 and transformed into E.coli via heat shock.</li>
 
<li>Single colonies were obtained by plating.</li>
 
<li>Single colonies were obtained by plating.</li>
<li>A colony PCR of Ni inducible promoter(pCPC-3301-Ni) was performed with 12 colonies.</li>
+
</div>
Two of the successful ones were used to inoculate overnight cultures.</li>
+
<br/>
<li>A colony PCR of pT-13-19-15 was performed with 7 colonies.</li>
+
  Two of the successful ones were used to inoculate overnight cultures.</li>
+
<li>Two kinds of plasmids were isolated using a miniprep kit.</li>
+
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.10th</b></h1>
 +
<div style="padding-left:32px;">
 +
<li>A colony PCR of Ni inducible promoter(pCPC-3301-Ni) was performed with 12 colonies.<li>
 +
&nbsp;&nbsp;Two of the successful ones were used to inoculate overnight cultures.<br/>
 +
<li>A colony PCR of pT-13-19-15 was performed with 7 colonies.<li>
 +
&nbsp;&nbsp;Two of the successful ones were used to inoculate overnight cultures.<br/>
 +
<br/>
  
         
+
<a href="https://static.igem.org/mediawiki/2016/8/81/Igem-6803-week4.png" data-lightbox="no" data-title=" ">
       
+
<img align="center" src="https://static.igem.org/mediawiki/2016/8/81/Igem-6803-week4.png"  alt="Igem-6803-week4" width="800" height="533"> <br/>
 +
</a>
 +
<br/>
 
</div>
 
</div>
            <a class="expand-btn4">Show More</a>
+
<br/>
  
  
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/igem.org/e/ec/T--Tianjin--cjw.jpg"  alt="IMG_2956" width="800" height="533"
+
</div>
</a>
+
<div id="Week5"></div>
 +
<a class="expand-btn4">Show More</a>
 +
 
 +
</div><!-- .entry-content -->
 +
 
 +
 
          
 
          
<hr class="article">
+
 
    </article>
 
    </article>
  
 +
<!------------------------------------week4 end------------------------------------------------>
  
  
  
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
+
 
<h1 class="entry-title">Week5(9/12/2016-9/18/2016)</h1>
+
<!------------------------------------week5 start------------------------------------------------>       
 +
 
 +
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<header class="entry-header">
 +
<h1 class="entry-title">Week5(9/11/2016-9/17/2016)</h1>
 +
</header><!-- .entry-header -->
 +
 
 
<div class="entry-content">
 
<div class="entry-content">
<p>
+
<div class="note-content4">
  
<li>Plasmids pT-13-19-15 were handed in for sequencing, which confirmed its correctness.</li>
 
<b>The sequencing results for both of them were error.</b>
 
<li>Colonies containing Ni inducible promoter were used to inoculate overnight cultures.</li>
 
<li>PCR was performed to check if the gene fragments were ligated correctly.</li>
 
    13_ fwd and 15_rev on pT-13-19-15<br/>
 
    Gel electrophoresis showed that it failed.<br/>
 
<li>Plasmids pCPC-3031-Ni were isolated using a miniprep kit.</li>
 
<li>Several PCRs were performed to check if the gene fragments were ligated correctly.</li>
 
1.13_fwd and 13_rev on pT-13-19-15<br/>
 
2.19_fwd and 19_rev on pT-13-19-15<br/>
 
3.15_fwd and 15_rev on pT-13-19-15<br/>
 
4.13_fwd and 19_rev on pT-13-19-15<br/>
 
5.19_fwd and 15_rev on pT-13-19-15<br/>
 
6.13_ wd and 15_rev on pT-13-19-15<br/>
 
    <b>The fourth and sixth ones were not successful.</b><br/>
 
<li><b>Repetition:</b>  Phosphorylated <i>13</i> was ligated into pT-19-15 and transformed into E.coli via heat shock.</li>
 
<li><b>Repetition:</b> Several PCRs were performed to check if the gene fragments were ligated correctly.</li>
 
1.13_fwd and 13_rev on pT-13-19-15<br/>
 
2.13_fwd and 19_rev on pT-13-19-15<br/>
 
<b>The second one was failed.</b>
 
  
  
 +
 +
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.11th</b></h1>
 +
<div style="padding-left:32px;"><li>Two kinds of plasmids were isolated using a miniprep kit.
 +
</li>
 +
</div>
 
<br/>
 
<br/>
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.14th</b></h1>
 +
<div style="padding-left:32px;"><li>The sequencing results for both of them were error.</li>
 +
</div>
 +
<br/>
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.15th</b></h1>
 +
<div style="padding-left:32px;"><li>Colonies containing Ni inducible promoter were used to inoculate overnight cultures.</li>
 +
<li>PCR was performed to check if the gene fragments were ligated correctly.</li>
 +
&nbsp;&nbsp;13_ fwd and 15_rev on pT-13-19-15<br/>
 +
<li>Gel electrophoresis showed that it failed.</li>
 +
</div>
 +
<br/>
  
  
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/igem.org/e/ec/T--Tianjin--cjw.jpg"  alt="IMG_2956" width="800" height="533"  
+
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.16th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids pCPC-3031-Ni were isolated using a miniprep kit.</li>
 +
</div>
 +
<br/>
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.17th</b></h1>
 +
<div style="padding-left:32px;">
 +
<li>Several PCRs were performed to check if the gene fragments were ligated correctly.</li>
 +
&nbsp;&nbsp;13_fwd and 13_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;19_fwd and 19_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;15_fwd and 15_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;13_fwd and 19_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;19_fwd and 15_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;13_ wd and 15_rev on pT-13-19-15<br/>
 +
<b>The fourth and sixth ones were not successful.</b><br/>
 +
<br/>
 +
 
 +
<a href="https://static.igem.org/mediawiki/2016/4/40/Igem-6803-week5.png" data-lightbox="no" data-title=" ">
 +
<img align="center"src="https://static.igem.org/mediawiki/2016/4/40/Igem-6803-week5.png"  alt="Igem-6803-week5" width="800" height="533" ><br/>
 
</a>
 
</a>
       
+
<br/>
<hr class="article">
+
<li><b>Repetition:</b>  Phosphorylated <i>13</i> was ligated into pT-19-15 and transformed into E.coli via heat shock.</li>
    </article>
+
</div>
 +
<br/>
  
  
Line 270: Line 425:
  
  
 +
</div>
 +
<div id="Week6"></div>
 +
<a class="expand-btn4">Show More</a>
 +
</div><!-- .entry-content -->
  
 +
 +
       
 +
 +
    </article>
  
 +
<!------------------------------------week5 end------------------------------------------------>
  
  
  
<!-- #post-4252 -->
+
<!------------------------------------week6 start------------------------------------------------>      
       
+
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
+
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<header class="entry-header">
 
<header class="entry-header">
<h1 class="entry-title">Week6(9/19/2016-9/25/2016)</h1>
+
<h1 class="entry-title">Week6(9/18/2016-9/24/2016)</h1>
 
</header><!-- .entry-header -->
 
</header><!-- .entry-header -->
  
 
<div class="entry-content">
 
<div class="entry-content">
<p>
+
 
<li>Medium preparation :BG-11.</li>
+
<div class="note-content4">
 +
 
 +
 
 +
 
 +
 
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.18th</b></h1>
 +
<div style="padding-left:32px;"><b>Repetition:</b> Several PCRs were performed to check if the gene fragments were ligated correctly.<br/>
 +
&nbsp;&nbsp;13_fwd and 13_rev on pT-13-19-15<br/>
 +
&nbsp;&nbsp;13_fwd and 19_rev on pT-13-19-15<br/>
 +
<b>The second one was failed.</b><br/>
 +
</div>
 +
<br/>
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.21th</b></h1>
 +
<div style="padding-left:32px;"><li>Medium preparation :BG-11.</li>
 
<li>19_ fwd and 15_rev were used to amplify <i>19-15</i>.</li>
 
<li>19_ fwd and 15_rev were used to amplify <i>19-15</i>.</li>
Gel electrophoresis showed that amplification of fragments was successfull.</li>
+
 
 +
</div>
 +
<br/>
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.22th</b></h1>
 +
<div style="padding-left:32px;">
 +
<li>Gel electrophoresis showed that amplification of fragments was successfull.</li>
 
<li>Ligated <i>13</i> and <i>19-15</i> via overlap PCR.</li>
 
<li>Ligated <i>13</i> and <i>19-15</i> via overlap PCR.</li>
This PCR worked well and the products were extracted from the gel using a Agarose Gel DNA Extration Kit.</li>
+
<li>This PCR worked well and the products were extracted from the gel using a Agarose Gel DNA Extration Kit.</li>
 
<li>Restriction digest on pCPC-3031-Ni with Sac I.</li>
 
<li>Restriction digest on pCPC-3031-Ni with Sac I.</li>
 +
<br/>
 +
<a href="https://static.igem.org/mediawiki/2016/8/89/Igem-6803-week6-2.jpg" data-lightbox="no" data-title=" ">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/8/89/Igem-6803-week6-2.jpg"  alt="Igem-6803-week6-1" width="300px">
 +
</a>
 +
 
<li>The fragment <i>13-19-15</i> was ligated onto T vector and transformed into E.coli via heat shock.</li>
 
<li>The fragment <i>13-19-15</i> was ligated onto T vector and transformed into E.coli via heat shock.</li>
<li>A colony PCR of pT-13-19-15 was performed with 12 colonies.</li>
+
 
Two of these colonies containing pT-13-19-15 were used to inoculate overnight cultures.</li>
+
<a href="https://static.igem.org/mediawiki/2016/0/06/Igem-6803-week6.jpg" data-lightbox="no" data-title=" ">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/0/06/Igem-6803-week6.jpg"  alt="Igem-6803-week6-2" width="300px" >
 +
</a>
 +
<br/>
 +
</div>
 +
<br/>
 +
 
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.23th</b></h1>
 +
<div style="padding-left:32px;"><li>A colony PCR of pT-13-19-15 was performed with 12 colonies.</li>
 +
<li>Two of these colonies containing pT-13-19-15 were used to inoculate overnight cultures.</li>
 
<li><i>13-19-15</i> gene fragment was phosphorylated.</li>
 
<li><i>13-19-15</i> gene fragment was phosphorylated.</li>
 
<li>Phosphorylated <i>13-19-15</i> was ligated into pCPC-3031-Ni and transformed into E.coli via heat shock.</li>
 
<li>Phosphorylated <i>13-19-15</i> was ligated into pCPC-3031-Ni and transformed into E.coli via heat shock.</li>
 +
</div>
 +
<br/>
  
<li>Plasmids pT-13-19-15 were isolated using a miniprep kit.</li>
 
<li>A colony PCR of pCPC-3031-Ni-13-19-15 was performed with 12 colonies.</li>
 
Three colonies were proved to be true. And two of them were used to inoculate overnight cultures.</li>
 
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.24th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids pT-13-19-15 were isolated using a miniprep kit.</li>
 +
</div>
 +
<br/>
  
 +
</div>
 +
<div id="Week7"></div>
 +
<a class="expand-btn4">Show More</a>
  
  
 +
</div><!-- .entry-content -->
  
<br />
+
 
+
 
+
 
+
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/igem.org/e/ec/T--Tianjin--cjw.jpg"  alt="IMG_2956" width="800" height="533"
+
</a>
+
 
          
 
          
<hr class="article">
+
 
    </article>
 
    </article>
  
 +
<!------------------------------------week6 end------------------------------------------------>
  
  
  
 +
<!------------------------------------week7 start------------------------------------------------>       
  
 +
        <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 +
<header class="entry-header">
 +
<h1 class="entry-title">Week7(9/25/2016-10/1/2016)</h1>
 +
</header><!-- .entry-header -->
  
 +
<div class="entry-content">
 +
<div class="note-content4">
 +
  
  
  
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.25th</b></h1>
 +
<div style="padding-left:32px;"><li>A colony PCR of pCPC-3031-Ni-13-19-15 was performed with 12 colonies.</li>
 +
<li>Three colonies were proved to be true. And two of them were used to inoculate overnight cultures.</li>
 +
<br/>
 +
<a href="https://static.igem.org/mediawiki/2016/2/2d/Igem-6803-week6-3.png" data-lightbox="no" data-title=" ">
 +
<img align="center" src="https://static.igem.org/mediawiki/2016/2/2d/Igem-6803-week6-3.png"  alt="Igem-6803-week6-3" width="800" height="533" ><br/>
 +
</a>
 +
<br/>
  
 +
</div>
 +
<br/>
  
  
  
 +
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.26th</b></h1>
 +
<div style="padding-left:32px;"><li>Plasmids pT-13-19-15 were handed in for sequencing, which confirmed its correctness.</li>
 +
<b>The sequencing results for them were correct.</b>
 +
<br/>
 +
</div>
 +
</br>
  
<article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173">
 
<header class="entry-header">
 
<h1 class="entry-title">Week7(9/26/2016-10/2/2016)</h1>
 
</header><!-- .entry-header -->
 
  
<div class="entry-content">
 
<p>
 
<li>Plasmids pT-13-19-15 were handed in for sequencing, which confirmed its correctness.</li>
 
<b>The sequencing results for them were correct.</b>
 
  
<br />
+
<b><h1 style="font-size:108%">&nbsp;&nbsp;Sep.28th</b></h1>
 +
<div style="padding-left:32px;"><li>We transformed the expression vector, pCPC-3031-Ni-13-19-15, into <i>Synechocystis 6803 </i>via electroporation.</li>
 +
<br/>
 +
<b>The story of 6803 is not over. Other team members will show the completed process during the presentation. </br>
 +
I will cherish the time spending with you for my whole life. ———by Jiawei Chen and Liangyu Qian</b>
 +
</div>
  
  
  
<img class="aligncenter size-full wp-image-4256" src="https://static.igem.org/mediawiki/igem.org/e/ec/T--Tianjin--cjw.jpg"  alt="IMG_2956" width="800" height="533"
+
</div>
</a>https://static.igem.org/mediawiki/2016/6/6d/Igem-6803-week3-1.jpg
+
<a class="expand-btn4">Show More</a>
<hr class="article">
+
 
    </article>
+
</div><!-- .entry-content -->
<!-- #post-4252 -->
+
 
           
+
 
          
 
          
 +
    </article>
 +
 +
<!------------------------------------week7 end------------------------------------------------>
  
  
  
<!-- #post-4176 -->
 
           
 
           
 
  
 
          
 
          
Line 367: Line 590:
  
 
</div>
 
</div>
<div class="side-nav">
+
 
<ul>
+
<li><a class="topLink" href="#Topp" style="color:#5555FF">Top</a></li>
+
                                                        <li><a class="topLink" href="#September" style="color:#5555FF">Week1</a></li>
+
<li><a class="topLink" href="#August" style="color:#5555FF">Week2</a></li>
+
<li><a class="topLink" href="#July" style="color:#5555FF">Week3</a></li>
+
<li><a class="topLink" href="#June" style="color:#5555FF">Week4</a></li>
+
<li><a class="topLink" href="#May" style="color:#5555FF">Week5</a></li>
+
<li><a class="topLink" href="#April" style="color:#5555FF">Week6</a></li>
+
<li><a class="topLink" href="#March" style="color:#5555FF">Week7</a></li>
+
</ul>
+
</div> 
+
  
  
Line 394: Line 606:
 
</div>
 
</div>
  
<div id="back-to-top" title="返回本页顶部" >
+
 
<svg id="rocket" version="1.1" xmlns="http://www.w3.org/2000/svg" width="32" height="32" viewBox="0 0 64 64">
+
        <path fill="#B6B6B6" d="M42.057,37.732c0,0,4.139-25.58-9.78-36.207c-0.307-0.233-0.573-0.322-0.802-0.329
+
        c-0.227,0.002-0.493,0.083-0.796,0.311c-13.676,10.31-8.95,35.992-8.95,35.992c-10.18,8-7.703,9.151-1.894,23.262
+
        c1.108,2.693,3.048,2.06,3.926,0.115c0.877-1.943,2.815-6.232,2.815-6.232l11.029,0.128c0,0,2.035,4.334,2.959,6.298
+
        c0.922,1.965,2.877,2.644,3.924-0.024C49.974,47.064,52.423,45.969,42.057,37.732z M31.726,23.155
+
        c-2.546-0.03-4.633-2.118-4.664-4.665c-0.029-2.547,2.012-4.587,4.559-4.558c2.546,0.029,4.634,2.117,4.663,4.664
+
        C36.314,21.143,34.272,23.184,31.726,23.155z"></path>
+
    </svg>
+
</div>
+
  
 
</body>
 
</body>
Line 415: Line 618:
 
<!-- Main JS -->
 
<!-- Main JS -->
 
 
   
 
    <script>
 
var x = 600;
 
var y = 2000;
 
for ( var i = 1; i < 22; i++ ){ 
 
var rand = parseInt(Math.random() * (x - y + 1) + y);
 
var randpic = "http://randomimage.setgetgo.com/get.php?width=" + rand;
 
    $("#MemberName" + i).attr("src", randpic);
 
}
 
    </script>
 
    <script type="text/javascript">
 
window._wpemojiSettings = {"baseUrl":"https:\/\/s.w.org\/images\/core\/emoji\/72x72\/","ext":".png","source":{"concatemoji":"http:\/\/www.camarts.cn\/wp-includes\/js\/wp-emoji-release.min.js?ver=4.5.3"}};
 
!function(a,b,c){function d(a){var c,d,e,f=b.createElement("canvas"),g=f.getContext&&f.getContext("2d"),h=String.fromCharCode;if(!g||!g.fillText)return!1;switch(g.textBaseline="top",g.font="600 32px Arial",a){case"flag":return g.fillText(h(55356,56806,55356,56826),0,0),f.toDataURL().length>3e3;case"diversity":return g.fillText(h(55356,57221),0,0),c=g.getImageData(16,16,1,1).data,d=c[0]+","+c[1]+","+c[2]+","+c[3],g.fillText(h(55356,57221,55356,57343),0,0),c=g.getImageData(16,16,1,1).data,e=c[0]+","+c[1]+","+c[2]+","+c[3],d!==e;case"simple":return g.fillText(h(55357,56835),0,0),0!==g.getImageData(16,16,1,1).data[0];case"unicode8":return g.fillText(h(55356,57135),0,0),0!==g.getImageData(16,16,1,1).data[0]}return!1}function e(a){var c=b.createElement("script");c.src=a,c.type="text/javascript",b.getElementsByTagName("head")[0].appendChild(c)}var f,g,h,i;for(i=Array("simple","flag","unicode8","diversity"),c.supports={everything:!0,everythingExceptFlag:!0},h=0;h<i.length;h++)c.supports[i[h]]=d(i[h]),c.supports.everything=c.supports.everything&&c.supports[i[h]],"flag"!==i[h]&&(c.supports.everythingExceptFlag=c.supports.everythingExceptFlag&&c.supports[i[h]]);c.supports.everythingExceptFlag=c.supports.everythingExceptFlag&&!c.supports.flag,c.DOMReady=!1,c.readyCallback=function(){c.DOMReady=!0},c.supports.everything||(g=function(){c.readyCallback()},b.addEventListener?(b.addEventListener("DOMContentLoaded",g,!1),a.addEventListener("load",g,!1)):(a.attachEvent("onload",g),b.attachEvent("onreadystatechange",function(){"complete"===b.readyState&&c.readyCallback()})),f=c.source||{},f.concatemoji?e(f.concatemoji):f.wpemoji&&f.twemoji&&(e(f.twemoji),e(f.wpemoji)))}(window,document,window._wpemojiSettings);
 
</script>
 
 
          
 
          
 
         <script>  /* show more */
 
         <script>  /* show more */
Line 491: Line 680:
  
 
         </script>
 
         </script>
 +
<script>  /* show more */
  
 +
      $(document).ready(function() {
 +
  $( '.expand-btn5' ).click(function() {
 +
var $text = $(this).html();
 +
$(this).siblings( '.note-content5' ).toggle();
 +
if( $text === 'Show More' ) {
 +
$(this).html( 'Show Less' );
 +
} else {
 +
$(this).html( 'Show More' );
 +
}
 +
});
 +
});
  
 +
        </script>
 +
<script>  /* show more */
 +
 +
      $(document).ready(function() {
 +
  $( '.expand-btn6' ).click(function() {
 +
var $text = $(this).html();
 +
$(this).siblings( '.note-content6' ).toggle();
 +
if( $text === 'Show More' ) {
 +
$(this).html( 'Show Less' );
 +
} else {
 +
$(this).html( 'Show More' );
 +
}
 +
});
 +
});
 +
 +
        </script>
  
 
          
 
          
Line 513: Line 730:
 
</html>
 
</html>
  
{{:Team:Tianjin/Templates/AddJS|:Team:Tianjin/Attribution/js/camarts.js}}
+
 
 +
{{:Team:Tianjin/Templates/Sponsor|}}

Latest revision as of 10:44, 5 November 2016

TEAM TIANJIN

LOGO


Team Tianjin-Attribution

Notes For Cyanobacteria

Week1(7/31/2016-8/6/2016)

  Jul.31th

  • Cultivation: 30µL mother liquid of Synechococcus sp PCC 7942 (wild type)were cultivated in 10 mL BG-11-media at 30°C and 140rpm.
  • The genome DNA of 7942 was extracted using a Genomic DNA Isolation Kit.

    • Show More

    Week2(8/14/2016-8/20/2016)

  • Synechococcus sp PCC 7942 had no signals of life.

    • Igem-6803-week2
    Show More

    Week3(8/28/2016-9/3/2016)

      Aug.29th

  • pMV-G19 and pMV-G15 containing our target genes were received.

    • Igem-6803-week3-1
  • Colonies were used to inoculate overnight cultures.

    •   Aug.30th

  • Plasmids were isolated using a miniprep kit.
  • Amplification of 19 and 15 with Q5 High-Fidelity DNA Polymerase out of E.coli.
    •   19 amplification at 65.0°C with 19.rev/fwd primes.
            PCR worked, positive control worked, no amplification of 19.
      15 amplification at 65.0°C with 15.rev/fwd primes.
            PCR worked, positive control worked, no amplification of 15.
  • A product length of 900 bp was expected. The gel shows that most plasmids seem to be correct.
    •   This result was confirmed by sequencing.
  • The fragments of 19 and 15 were purified with PCR Purification Kit.

    •   Aug.31th

  • Ligation of 15 with 19.
  • We add a single 3`-adenine overhang to each end of the fragment of 19 and then purified with DNA Purification Kit.
  • 19 was ligated into T vectors via TA clone and transformed into E.coli via heat shock.

    •   Sep.1th

  • A colony PCR was performed with five colonies.
  • Gel electrophoresis showed that 5 colonies were positive for insertion of 19.
  • Two of these colonies containing 19 were used to inoculate overnight cultures.
  • 15 gene fragment was phosphorylated.

    •   Sep.2th

  • Plasmids containing T vector with 19(pT-19)were isolated using a miniprep kit.
  • Mono-restriction digest of pT-19 with stu I.
  • The enzyme-digested product was dephosphorylation.

    • Igem-6803-week3-2
  • Dephosphorylated plasmid and phosphorylated gene 15 were connected.
  • Ligation product was transformed into E.coli via heat shock.

    •   Sep.3th

  • A colony PCR was performed with twelve colonies.
  • Gel electrophoresis showed that 2 colonies were positive for connecting the plasmid and gene fragment.
  • These two colonies were used to inoculate overnight cultures.

    • Show More

    Week4(9/4/2016-9/10/2016)

      Sep.4th

  • Plasmids with correct sequence of 19-15 were isolated using a miniprep kit.
  • Mono-restriction digest of pT-19-15 with Nru I.
  • The enzyme-digested product was dephosphorylation.

    •   Sep.6th

  • Colonies containing gene 13 were used to inoculate overnight cultures.

    •   Sep.7th

  • Plasmids were isolated using a miniprep kit.
  • Amplification of 13 with Q5 High-Fidelity DNA Polymerase out of E.coli
  • 13 amplification at 65.0°C with 13.rev/fwd primes
    •   PCR worked, positive control worked, no amplification of 13
  • The fragments of 13 were purified with PCR Purification Kit.

    •   Sep.8th

  • 13 gene fragment was phosphorylated.

    •   Sep.9th

  • Insertion of Ni promoter and ligation of 13-19-15
  • Ni inducible promoter was ligated into pCPC-3301 vector.
  • Phosphorylated 13 was ligated into pT-19-15 and transformed into E.coli via heat shock.
  • Single colonies were obtained by plating.

    •   Sep.10th

  • A colony PCR of Ni inducible promoter(pCPC-3301-Ni) was performed with 12 colonies.
  •   Two of the successful ones were used to inoculate overnight cultures.
  • A colony PCR of pT-13-19-15 was performed with 7 colonies.
  •   Two of the successful ones were used to inoculate overnight cultures.

    Igem-6803-week4


    • Show More

    Week5(9/11/2016-9/17/2016)

      Sep.11th

  • Two kinds of plasmids were isolated using a miniprep kit.

    •   Sep.14th

  • The sequencing results for both of them were error.

    •   Sep.15th

  • Colonies containing Ni inducible promoter were used to inoculate overnight cultures.
  • PCR was performed to check if the gene fragments were ligated correctly.
    •   13_ fwd and 15_rev on pT-13-19-15
  • Gel electrophoresis showed that it failed.

    •   Sep.16th

  • Plasmids pCPC-3031-Ni were isolated using a miniprep kit.

    •   Sep.17th

  • Several PCRs were performed to check if the gene fragments were ligated correctly.
    •   13_fwd and 13_rev on pT-13-19-15
      19_fwd and 19_rev on pT-13-19-15
      15_fwd and 15_rev on pT-13-19-15
      13_fwd and 19_rev on pT-13-19-15
      19_fwd and 15_rev on pT-13-19-15
      13_ wd and 15_rev on pT-13-19-15
    The fourth and sixth ones were not successful.

    Igem-6803-week5
  • Repetition: Phosphorylated 13 was ligated into pT-19-15 and transformed into E.coli via heat shock.

    • Show More

    Week6(9/18/2016-9/24/2016)

      Sep.18th

    Repetition: Several PCRs were performed to check if the gene fragments were ligated correctly.
      13_fwd and 13_rev on pT-13-19-15
      13_fwd and 19_rev on pT-13-19-15
    The second one was failed.

      Sep.21th

  • Medium preparation :BG-11.
  • 19_ fwd and 15_rev were used to amplify 19-15.

    •   Sep.22th

  • Gel electrophoresis showed that amplification of fragments was successfull.
  • Ligated 13 and 19-15 via overlap PCR.
  • This PCR worked well and the products were extracted from the gel using a Agarose Gel DNA Extration Kit.
  • Restriction digest on pCPC-3031-Ni with Sac I.

    • Igem-6803-week6-1
  • The fragment 13-19-15 was ligated onto T vector and transformed into E.coli via heat shock.
    • Igem-6803-week6-2

      Sep.23th

  • A colony PCR of pT-13-19-15 was performed with 12 colonies.
  • Two of these colonies containing pT-13-19-15 were used to inoculate overnight cultures.
  • 13-19-15 gene fragment was phosphorylated.
  • Phosphorylated 13-19-15 was ligated into pCPC-3031-Ni and transformed into E.coli via heat shock.

    •   Sep.24th

  • Plasmids pT-13-19-15 were isolated using a miniprep kit.

    • Show More

    Week7(9/25/2016-10/1/2016)

      Sep.25th

  • A colony PCR of pCPC-3031-Ni-13-19-15 was performed with 12 colonies.
  • Three colonies were proved to be true. And two of them were used to inoculate overnight cultures.

    • Igem-6803-week6-3

      Sep.26th

  • Plasmids pT-13-19-15 were handed in for sequencing, which confirmed its correctness.
    • The sequencing results for them were correct.

      Sep.28th

  • We transformed the expression vector, pCPC-3031-Ni-13-19-15, into Synechocystis 6803 via electroporation.

    • The story of 6803 is not over. Other team members will show the completed process during the presentation.
    I will cherish the time spending with you for my whole life. ———by Jiawei Chen and Liangyu Qian
    Show More
    info_outline
    Notice: This page is currently under construction. Contents in this page are temporaory and will be modified several times before the final release.     — 2016 iGEM Team Tianjin


    Team Tianjin Sponsor Alltech
    Team Tianjin Sponsor GenScript
    Team Tianjin Sponsor SynbioTech