Team:Braunschweig/Notebook

From 2013.igem.org

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<b>Investigators: Kevin, Kerstin, Laura</b><br>
<b>Investigators: Kevin, Kerstin, Laura</b><br>
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We prepared some chemically competent <i>E. coli</i> XL1Blue MRF cells for all the transformations we are going to perform during the project.</p>
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We prepared some chemically competent <i>E. coli</i> XL1Blue MRF' cells for all the transformations we are going to perform during the project.</p>
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<b>Investigators: Kevin, Kerstin, Laura</b><br>
<b>Investigators: Kevin, Kerstin, Laura</b><br>
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Cells from yesterday's transformation only grew on agar plates containing ampicillin. The plates with the additional antibiotics were empty, thus we can conclude that our competent <i>E. coli</i> XL1Blue MRF cells do not carry other antibiotic resistances.<br>
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Cells from yesterday's transformation only grew on agar plates containing ampicillin. The plates with the additional antibiotics were empty, thus we can conclude that our competent <i>E. coli</i> XL1 Blue MRF' cells do not carry other antibiotic resistances.<br>
111 colonies were counted for pUC18 transformation, 50 for pUC19 transformation on ampicillin containing agar plates. According to these numbers the transformation Efficiency was calculated.<br>
111 colonies were counted for pUC18 transformation, 50 for pUC19 transformation on ampicillin containing agar plates. According to these numbers the transformation Efficiency was calculated.<br>
Transformation efficiency:<br>  
Transformation efficiency:<br>  
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   <div id="Week2" class="menuSection">
   <div id="Week2" class="menuSection">
     <h2><a href="#Week2">Week 2: May 27 - June 1, 2013</a></h2>
     <h2><a href="#Week2">Week 2: May 27 - June 1, 2013</a></h2>
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     <p style="margin-left:5px; margin-right:5px;">The distribution kit arrived and we started with the actual labwork. 19 BioBricks had to be transformed into our <i>E. coli</i> strain to secure the parts. Additionally we developed the cloning strategy for the next weeks.</p>
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     <p style="margin-left:5px; margin-right:5px;">The distribution kit arrived and we started with the actual labwork. 19 BioBricks had to be transformed into our <i>E. coli</i> XL1 Blue MRF' strain to secure the parts. Additionally we developed the cloning strategy for the next weeks.</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">Monday, May 27, 2013</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">Monday, May 27, 2013</p>
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<b>Investigators: Laura, Kerstin</b><br>
<b>Investigators: Laura, Kerstin</b><br>
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We received the new set of BioBricks we ordered from the registry: B0015 (this one is going to be our new terminator, replacing the combination of B0010 and B0012), B0017, E0420, J23100, J23106. These were transformed via heatshock in <i>E. coli</i> XL1Blue MRF cells. We also prepared following of the miniprepped BioBricks for sequencing:  C0061, B0012, B1009. The results are outlined in the following table:  
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We received the new set of BioBricks we ordered from the registry: B0015 (this one is going to be our new terminator, replacing the combination of B0010 and B0012), B0017, E0420, J23100, J23106. These were transformed via heatshock in <i>E. coli</i> XL1 Blue MRF' cells. We also prepared following of the miniprepped BioBricks for sequencing:  C0061, B0012, B1009. The results are outlined in the following table:  
<img alt="June4" src="https://static.igem.org/mediawiki/2013/f/fd/Braunschweig_Labjournal_June4.png" width="600" align="center" vspace="0" hspace="20"/>
<img alt="June4" src="https://static.igem.org/mediawiki/2013/f/fd/Braunschweig_Labjournal_June4.png" width="600" align="center" vspace="0" hspace="20"/>
</p>
</p>
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<b>Investigators: Laura, Oliver, Jan </b><br>
<b>Investigators: Laura, Oliver, Jan </b><br>
Today, we digested the inducible promoters, followed by purification and clean-up. Then we equipped the inducible and previously digested constitutive promoters with a RBS (B0032) by ligating respective parts. Subsequently, these ligated constructs were used to transform competent bacteria.
Today, we digested the inducible promoters, followed by purification and clean-up. Then we equipped the inducible and previously digested constitutive promoters with a RBS (B0032) by ligating respective parts. Subsequently, these ligated constructs were used to transform competent bacteria.
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We also inoculated overnight suspension cultures with B0015- and B0032-transformed <i>E. coli</i> cells from glycerol stocks for DNA preparation.</p>
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We also inoculated overnight suspension cultures with B0015- and B0032-transformed <i>E. coli</i> XL1 Blue MRF' cells from glycerol stocks for DNA preparation.</p>
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<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>
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Yesterday's ligations transformed into <i>E. coli</i> XL1 by heatshock and plated on 2xYT agar containing glucose and Chloramphenicol.<br>  
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Yesterday's ligations transformed into <i>E. coli</i> XL1 MRF' by heatshock and plated on 2xYT agar containing glucose and Chloramphenicol.<br>  
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Since the chromoprotein DNA from Uppsala iGEM Team 2011 arrived today we now switched to our new cloning strategy starting with resuspending and transforming the newly arrived DNA into <i>E. coli</i> XL1 by heatshock. Cells were as well plated on 2xYT agar containing Glucose and Chloramphenicol.<br>
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Since the chromoprotein DNA from Uppsala iGEM Team 2011 arrived today we now switched to our new cloning strategy starting with resuspending and transforming the newly arrived DNA into <i>E. coli</i> XL1Blue MFR' by heatshock. Cells were as well plated on 2xYT agar containing glucose and chloramphenicol.<br>
Even if we switched to our new strategy we still kept working on the fluorescence markers. Therefore we digested the BioBricks E0420 (eCFP), E0430 (YFP) and J06702 (mCherry) as well as our promotor-RBS-LasR and promotor-RBS-RhlR-constructs. Still lacking the construct containing LuxR we decided to proceed with the promotor-RBS-construct instead to ligate it to the YFP-Brick. Gel extraction was performed for the inserts and DNA purification for the vector parts. Inserts and bricks were ligated overnight using T4 DNA ligase (NEB) at 16°C.<br><br>
Even if we switched to our new strategy we still kept working on the fluorescence markers. Therefore we digested the BioBricks E0420 (eCFP), E0430 (YFP) and J06702 (mCherry) as well as our promotor-RBS-LasR and promotor-RBS-RhlR-constructs. Still lacking the construct containing LuxR we decided to proceed with the promotor-RBS-construct instead to ligate it to the YFP-Brick. Gel extraction was performed for the inserts and DNA purification for the vector parts. Inserts and bricks were ligated overnight using T4 DNA ligase (NEB) at 16°C.<br><br>
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Since we now have our first constructs containing the inducible promotors as well as the the Ampicillin resistence gen we started our first leakiness experiments. All constructs (P<sub>las</sub>, P<sub>rhl</sub>, P<sub>lux</sub> in combination with the RBS and <i>ampR</i>) were cultivated overnight in 2xYT medium containing various Ampicillin concentrations.</p>
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Since we now have our first constructs containing the inducible promotors as well as the the Ampicillin resistence gen we started our first leakiness experiments. All constructs (P<sub>las</sub>, P<sub>rhl</sub>, P<sub>lux</sub> in combination with the RBS and <i>ampR</i>) were cultivated overnight in 2xYT medium containing various ampicillin concentrations.</p>
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<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>
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Before we started working on our own chromoprotein-constructs, we screened for the optimum cultivation conditions. We cultivated <i>E. coli</i> 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. These experiments led to the conclusion that low oxygen supply and a temperature of 37°C result in higher expression rates.<br><br>
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Before we started working on our own chromoprotein-constructs, we screened for the optimum cultivation conditions. We cultivated <i>E. coli</i> XL1 Blue MRF' 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. These experiments led to the conclusion that low oxygen supply and a temperature of 37°C result in higher expression rates.<br><br>
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The evaluation of the leakiness of the inducible promotors showed that only the P<sub>rhl</sub> is not leaky. P<sub>lux</sub> as well as P<sub>las</sub> were leaky and showed growth of <i>E. coli</i> XL1 at all tested Ampicillin concentrations. Therefore we repeated the experiment using higher Ampicillin conentrations.<br><br>
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The evaluation of the leakiness of the inducible promotors showed that only the P<sub>rhl</sub> is not leaky. P<sub>lux</sub> as well as P<sub>las</sub> were leaky and showed growth of <i>E. coli</i> XL1 Blue MRF' at all tested Ampicillin concentrations. Therefore we repeated the experiment using higher Ampicillin conentrations.<br><br>
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The bricks containing the fluorescencw markers ligated yesterday were transformed in <i>E. coli</i> XL1 by heatshock.<br><br>
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The bricks containing the fluorescencw markers ligated yesterday were transformed in <i>E. coli</i> XL1 Blue MRF' by heatshock.<br><br>
<img alt="July3" src="https://static.igem.org/mediawiki/2013/f/fa/Braunschweig_Lab_Journal_July_3.png" width="200" align="right" vspace="0" hspace="10"/>Colony PCR of the constructs containing lactonase and LuxI which were transformed yesterday was performed. Since all screened colonies showed religated vectors we decided to try an alternative restriction strategy to combine the BioBricks by using the endonuclease NcoI.<br>   
<img alt="July3" src="https://static.igem.org/mediawiki/2013/f/fa/Braunschweig_Lab_Journal_July_3.png" width="200" align="right" vspace="0" hspace="10"/>Colony PCR of the constructs containing lactonase and LuxI which were transformed yesterday was performed. Since all screened colonies showed religated vectors we decided to try an alternative restriction strategy to combine the BioBricks by using the endonuclease NcoI.<br>   
B0032, C0060 and C0061-B0015 were digested with NcoI and corresponding SpeI and XbaI. Gel extraction was performed for the vector DNA as well as the inserts.<br>
B0032, C0060 and C0061-B0015 were digested with NcoI and corresponding SpeI and XbaI. Gel extraction was performed for the vector DNA as well as the inserts.<br>
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Overnight liquid cultures were inoculated with <i>E. coli</i> XL1 containing the chromoprotein in 2xYT supplemented with Chloramphenicol.</p>  
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Overnight liquid cultures were inoculated with <i>E. coli</i> XL1 Blue MRF' containing the chromoprotein in 2xYT supplemented with chloramphenicol.</p>  
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<b>Investigators: Kerstin, Laura </b><br>
<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="150" align="right" vspace="0" hspace="10"/>
<img alt="July4" src="https://static.igem.org/mediawiki/2013/1/1a/Braunschweig_Lab_Journal_July_4_1.png" width="150" align="right" vspace="0" hspace="10"/>
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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 <i>E. coli</i> XL1 by heatshock and plated on agar plates.<br>
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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 <i>E. coli</i> XL1 Blue MRF' 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><br><br><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><br><br><br>
<img alt="July4_2" src="https://static.igem.org/mediawiki/2013/b/b4/Braunschweig_Lab_Journal_July_4_2.png" width="150" align="right" vspace="0" hspace="10"/>The chromoprotein cultures were miniprepped and DNA was directly used for digestion to combine the chromoproteins with our promotor-RBS construct. The insert parts were extracted from an agarose gel while the vector part was dephosphorylated and purified using DNA clean-up columns.<br>  
<img alt="July4_2" src="https://static.igem.org/mediawiki/2013/b/b4/Braunschweig_Lab_Journal_July_4_2.png" width="150" align="right" vspace="0" hspace="10"/>The chromoprotein cultures were miniprepped and DNA was directly used for digestion to combine the chromoproteins with our promotor-RBS construct. The insert parts were extracted from an agarose gel while the vector part was dephosphorylated and purified using DNA clean-up columns.<br>  
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<b>Investigators: Kerstin, Laura, Jan </b><br>
<b>Investigators: Kerstin, Laura, Jan </b><br>
When we checked the agar plates for transformed colonies with the LuxI and lactonase containing constructs we did not have any colonies.<br>  
When we checked the agar plates for transformed colonies with the LuxI and lactonase containing constructs we did not have any colonies.<br>  
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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 <i>E. coli</i> XL1 by heatshock and plated on agar plates. We cannot wait to see colorful colonies on Sunday :-)<br><br>
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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 <i>E. coli</i> XL1 Blue MRF' 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>
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 leakiness of the P<sub>las</sub> and P<sub>lux</sub> 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>   
A new idea to cope with the leakiness of the P<sub>las</sub> and P<sub>lux</sub> 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>   
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<b>Investigators: Roman </b><br>
<b>Investigators: Roman </b><br>
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We prepared pre-cultures of our chromoprotein expression cassettes (promoter-RBS-chromoprotein) in E. coli XL1. For each chromoprotein (amilGFP, eforRed, aeBlue) 50 ml 2xYT containing chloramphenicol were inoculated from -80°C glycerol stocks and grown at 37°C and 250 rpm over night.<br></p>
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We prepared pre-cultures of our chromoprotein expression cassettes (promoter-RBS-chromoprotein) in E. coli XL1 Blue MRF'. For each chromoprotein (amilGFP, eforRed, aeBlue) 50 ml 2xYT containing chloramphenicol were inoculated from -80°C glycerol stocks and grown at 37°C and 250 rpm over night.<br></p>
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During the day we noticed that the 2xYT medium used for the pre-cultures yesterday showed contamination. Thus, there is a high possibility  of contamination in the pre-culture as well as in the main culture. Therefore we decided to repeat the experiment. New pre-cultures of the three chromoprotein expression cassettes where inoculated in 50 ml 2xYT containing chloramphenicol directly from -80°C.<br>
During the day we noticed that the 2xYT medium used for the pre-cultures yesterday showed contamination. Thus, there is a high possibility  of contamination in the pre-culture as well as in the main culture. Therefore we decided to repeat the experiment. New pre-cultures of the three chromoprotein expression cassettes where inoculated in 50 ml 2xYT containing chloramphenicol directly from -80°C.<br>
In order to have our constructs available in different E. coli strains for the fluorescence microscopy experiments, the eforRed expression cassette was transformed into <i>E. coli</i> Top10F' by electroporation. Transformed cells were plated on 2xYT agar containing chloramphenicol and incubated over night at 37°C.<br>
In order to have our constructs available in different E. coli strains for the fluorescence microscopy experiments, the eforRed expression cassette was transformed into <i>E. coli</i> Top10F' by electroporation. Transformed cells were plated on 2xYT agar containing chloramphenicol and incubated over night at 37°C.<br>
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A continuous cultivation of the Rhl inducible construct in E. coli Top 10 prepared, including preparation of pre-cultures of our inducible construct in 50 ml 2xYT containing chloramphenicol and grown at 37°C and 250 rpm over night.<br>
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A continuous cultivation of the Rhl inducible construct in E. coli Top10F' prepared, including preparation of pre-cultures of our inducible construct in 50 ml 2xYT containing chloramphenicol and grown at 37°C and 250 rpm over night.<br>
  </p>
  </p>
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<b>Investigators: Anna, Kevin </b><br>
<b>Investigators: Anna, Kevin </b><br>
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Transformation of the eforRed expression cassette in <i>E. coli</i> Top10 was performed by electroporation.<br>  
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Transformation of the eforRed expression cassette in <i>E. coli</i> Top10F' was performed by electroporation.<br>  
The reporter strains for the Las and Rhl systems (<i>E. coli</i> JM109 pSB1075 and <i>E. coli</i> JM109 pSB406 respectively) arrived today. Liquid cultures in 2xYT containing ampicillin were inoculated and grown at 37°C and 250 rpm overnight.<br>  
The reporter strains for the Las and Rhl systems (<i>E. coli</i> JM109 pSB1075 and <i>E. coli</i> JM109 pSB406 respectively) arrived today. Liquid cultures in 2xYT containing ampicillin were inoculated and grown at 37°C and 250 rpm overnight.<br>  
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Pre-cultures of <i>E. coli</i> Top10F’ containing final P<sub>Rhl</sub> inducible construct and <i>E. coli</i> XL1 containing final P<sub>Las</sub> inducible construct in 50 ml 2xYT containing chloramphenicol for continuous cultures were grown at 37°C and 250 rpm overnight.<br></p>  
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Pre-cultures of <i>E. coli</i> Top10F' containing final P<sub>Rhl</sub> inducible construct and <i>E. coli</i> XL1 Blue MRF' containing final P<sub>Las</sub> inducible construct in 50 ml 2xYT containing chloramphenicol for continuous cultures were grown at 37°C and 250 rpm overnight.<br></p>  
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<b>Investigators: Laura, Kerstin, Roman, Kevin, Jan, Judith </b><br>
<b>Investigators: Laura, Kerstin, Roman, Kevin, Jan, Judith </b><br>
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Pre-culture of erforRed expression cassette in <i>E. coli</i> Top10F’ in 50 ml 2xYT containing Chloramphenicol was inoculated from the  agar plate and grown at 37°C and 250 rpm overnight.<br>
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Pre-culture of erforRed expression cassette in <i>E. coli</i> Top10F' in 50 ml 2xYT containing chloramphenicol was inoculated from the  agar plate and grown at 37°C and 250 rpm overnight.<br>
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For the reproduction of the growth curve a pre-culture of the Rhl inducible construct in <i>E. coli</i> Top10 in 30 mL 2xYT containing Chloramphenicol and incubated at 37°C overnight. <br>
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For the reproduction of the growth curve a pre-culture of the Rhl inducible construct in <i>E. coli</i> Top10F' in 30 mL 2xYT containing Chloramphenicol and incubated at 37°C overnight. <br>
To test the production of AHLs by our final constructs we prepared a pre-culture of each reporter strain in 30 ml 2xYT containing Ampicillin and incubated them overnight at 37°C and 250 rpm. We also made glycerol cell stocks of the reporter strains.<br>
To test the production of AHLs by our final constructs we prepared a pre-culture of each reporter strain in 30 ml 2xYT containing Ampicillin and incubated them overnight at 37°C and 250 rpm. We also made glycerol cell stocks of the reporter strains.<br>

Revision as of 17:35, 3 October 2013

Labjournal

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This is the documentation of our lab work. An overview on how we approached this project can be found under Approach. 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.

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