Difference between revisions of "Team:TCU Taiwan/Result/vitro"

Line 11: Line 11:
 
         position:static;
 
         position:static;
 
width:100%;
 
width:100%;
 +
z-index:1;
 +
        overflow:visible;
 +
        margin-bottom:2%;
 +
        display: inline-block
 +
}
 +
#form1 {
 +
        position:static;
 +
width:90%;
 
z-index:1;
 
z-index:1;
 
         overflow:visible;
 
         overflow:visible;
Line 19: Line 27:
 
<body>
 
<body>
 
<img src="https://static.igem.org/mediawiki/2015/1/16/2015tcutaiwanResult.jpg" width="100%" align="center"/><br>
 
<img src="https://static.igem.org/mediawiki/2015/1/16/2015tcutaiwanResult.jpg" width="100%" align="center"/><br>
  <div id="form" style="background: rgba(100%,100%,100%,0.5); overflow-x:hidden;overflow-y:hidden; ">
+
  <div id="form1" style="background: rgba(100%,100%,100%,0.5); overflow-x:hidden;overflow-y:hidden; ">
  
 
<h1>
 
<h1>

Revision as of 15:39, 12 September 2015


Aug. 6th ,2015

•  * PCR signiferin
2% gel. The PCR product of signiferin should be 100~200 bp. As the result, there is band between 100~200 bp on sample 2 so we consider it is correct.

Aug. 15th ,2015

•  signiferin TA plasmid purification

0.8% gel. The size of TA plasmid with signiferin insert should be 2000~3000 bp. In addition, plasmid will become sorpercoil so it will run faster. Therefore, we consider these are the correct plasmid.


Aug. 16th ,2015

•  pQE60 plasmid digest with enzyme BamH I and Nco I biobrick digest with enzyme EcoRI and Pst I

2% gel. The size of signiferin insert should be 100~20 bp. In addition, the signiferin insert in biobrick should be a little bigger than in pQE60. As the result, these two are all the correct sample we need.


Aug. 21st ,2015

•  PCR Epi-1 insert
2% gel. It is the correct size that Epi-1 PCR product have band between 200~300 bp. But, there is also band on blank. We consider it was polluted when we add reagent.
•  plasmid purification of pQE60 vector with signiferin insert
0.8% gel. The size of our plasmid should be 3000 to 4000. As the result, these samples are the plasmid we need.

Aug. 22rd ,2015

•  Plasmid purification of pQE60 plasmid with signiferin insert
•  Plasmid purification of backbone with signiferin insert
0.8% gel. The size of signiferin biobrick should be 2000~3000 bp, and the size of pQE60 plasmid with signiferin should be 3000~4000 bp. In addition, the plasmid will become surpercoil so it will run faster. Therefore, they are all correct pasmid.

Aug. 23rd ,2015

•  Enzyme digestion to check the clone of biobrick with signiferin
2% gel. The size of signiferin insert should be 100 to 200 bp. There is band on the sample 2 of enzyme digest product. As the result, we can make sure that the signiferin has been ligated in backbone.



             
Flag Counter
Contact us
tcutaiwan@gmail.com
No.701, Sec. 3, Zhongyang Rd. Hualien 97004, Taiwan