Team:Ehime-Japan/Modeling

From 2012.igem.org

(Difference between revisions)
Line 129: Line 129:
<p>Method<p/>
<p>Method<p/>
<b>
<b>
 +
E.coli (pIJ106b, pJT122, plPCB) is cultivated in TY culture medium for 7 hours. It was precipitated by centrifugation and washed with 1 % NaClaq.
 +
400 &mu;L of 1% NaCl was added to the E.coli sample and protein synthesis was stopped by addition of tetracyclin at the concentration of 100 &mu;g/mL.
 +
An aliquot from each sample was plated on agar and cultured overnight.
 +
The solution was exposed to blue LED light, and we took a color picture every 1 hour for 6 hours.
 +
By using the ImageJ software, we measured the intensity of light from GFP.
 +
</body>
</body>
</html>
</html>

Revision as of 03:10, 27 September 2012

Ehime-Japan iGEM Team: Welcome


Introduction

In our experiment of the E.co-mail, the important thing is to degrade GFP-Lon-tag more rapidly. GFP is usually stable and has a long half–life. So, we thought of how to measure the reaction rate.

Method

E.coli (pIJ106b, pJT122, plPCB) is cultivated in TY culture medium for 7 hours. It was precipitated by centrifugation and washed with 1 % NaClaq. 400 μL of 1% NaCl was added to the E.coli sample and protein synthesis was stopped by addition of tetracyclin at the concentration of 100 μg/mL. An aliquot from each sample was plated on agar and cultured overnight. The solution was exposed to blue LED light, and we took a color picture every 1 hour for 6 hours. By using the ImageJ software, we measured the intensity of light from GFP.