Team:Braunschweig/Notebook
From 2013.igem.org
(Difference between revisions)
Line 376: | Line 376: | ||
<p><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px"> | <p><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px"> | ||
<b>Investigators: Kerstin, Laura </b><br> | <b>Investigators: Kerstin, Laura </b><br> | ||
- | + | Before we started working on our own chromoprotein-constructs, we screened for the optimum cultivation conditions. We cultivated E. coli XL1 containing a new construct from Uppsala iGEM containing the device J23110-B0034-aeBlue. We tested expression of the blue chromoprotein at different temperatures, oxygen supply and rpm. From that experiments we came to the conclusion that low oxygen supply and a temperature of 37°C leads to higher expression rates.<br><br> | |
The evaluation of the experiment for the inducible promotors showed that only the Prhl is not leaky. Plux as well as Plas were leaky and showed growth of E. coli XL1 at all tested ampicillin concentrations. Therefore we repeated the experiment using higher ampicillin conentrations.<br><br> | The evaluation of the experiment for the inducible promotors showed that only the Prhl is not leaky. Plux as well as Plas were leaky and showed growth of E. coli XL1 at all tested ampicillin concentrations. Therefore we repeated the experiment using higher ampicillin conentrations.<br><br> | ||
Line 386: | Line 386: | ||
Overnight liquid cultures were inoculated with E. coli XL1 containing the chromoprotein in 2xYT containing chloramphenicol.</p> | Overnight liquid cultures were inoculated with E. coli XL1 containing the chromoprotein in 2xYT containing chloramphenicol.</p> | ||
+ | <p><p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Thursday, July 4, 2013</p> | ||
+ | <p><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px"> | ||
+ | <b>Investigators: Kerstin, Laura </b><br> | ||
+ | <img alt="July4" src="https://static.igem.org/mediawiki/2013/1/1a/Braunschweig_Lab_Journal_July_4_1.png" width="200" align="right" vspace="0" hspace="10"/> | ||
+ | Ligation of the constructs B0032-C0060 (containing lactonase) and B0032-C0061-B0015 (containing LuxI) was performed for 30 minutes at room temperature using T4 DNA Ligase (NEB). Constructs were transformed in E. coli XL1 by heatshock and plated on agar plates.<br> | ||
+ | As we were still having trouble with the brick C0062 (LuxR) we amplified the brick from the device F2620 using Q5 Polymerase (NEB). Gelextraction was performed for the PCR products.<br><br> | ||
+ | |||
+ | <img alt="July4" src="https://2013.igem.org/File:Braunschweig_Lab_Journal_July_4_2.png" width="200" align="right" vspace="0" hspace="10"/>The chromoprotein cultures were minipreped and DNA was directly used for digestion to combine the chromoproteins with our promotor-RBS construct. The insert parts were extracted from agarose gel while the vector part was dephosphorylated and purified using DNA clean-up columns.<br> | ||
+ | Colony PCR was conducted for the constructs with the fluorescent proteins which were transformed yesterday. We were able to identify colonies with the right brick size for all tested constructs.</p> | ||
+ | |||
+ | <p><p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Friday, July 5, 2013</p> | ||
+ | <p><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px"> | ||
+ | <b>Investigators: Kerstin, Laura, Jan </b><br> | ||
+ | Checking the agar plates for transformed colonies with the LuxI and lactonase containing constructs we did not have any colonies.<br> | ||
+ | The digested chromoprotein DNA was ligated with the RBS and the promotor-RBS construct at room temperature for 30 minutes. The ligated DNA was transformed in E. coli XL1 by heatshock and plated on agar plates. We cannot wait to see colorful colonies on Sunday :-)<br><br> | ||
+ | Since we almost ran out off our competent cells it was time for new ones. New compentent cells were made and transformation efficiency was tested.<br> | ||
+ | A new idea to cope with the leakyness of the Plas and Plux was to try a different antibiotic which cannot be metabolised. We used carbenicillin instead of ampicillin at different concentrations in liquid culture with 2xYT medium. Unfortunatly no effect could be observed on the leakyness of both inducible promotors.</p> | ||
</div> | </div> |
Revision as of 23:17, 17 September 2013
Labjournal
This is the documentation of our lab work. For detailed protocols of certain procedures please refer to Protocols. Attributions are given for each day, however please check our Attributions section for efforts beyond the lab work.
Our sponsors