Team:Toulouse/Notebook/Protocols

From 2014.igem.org

(Difference between revisions)
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<p class="title2">First step</p>
<p class="title2">First step</p>
<p class="title3">Both parts have the same antibiotic resistance</p>
<p class="title3">Both parts have the same antibiotic resistance</p>
-
<p class="texte">1) Digestion mix
+
<p class="texte"><b>1) Digestion mix</b>
<br> For the vector :
<br> For the vector :
<br>- 5 µL of miniprep plasmid  
<br>- 5 µL of miniprep plasmid  
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- Incubate 15 minutes at 37°C  
- Incubate 15 minutes at 37°C  
-
<br><br>2) Gel extraction
+
<br><br><b>2) Gel extraction</b>
<br>
<br>
- Prepare a 1% or 2% electrophoresis agarose gel with 0.5x TAE buffer
- Prepare a 1% or 2% electrophoresis agarose gel with 0.5x TAE buffer
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<p class="title3">The two parts have a different antibiotic resistance</p>
<p class="title3">The two parts have a different antibiotic resistance</p>
-
<p class="texte">1) Digestion mix  
+
<p class="texte"><b>1) Digestion mix</b>
<br>For each part, add :  
<br>For each part, add :  
<br>- 5 µL of miniprep plasmid  
<br>- 5 µL of miniprep plasmid  
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<p class="texte">
<p class="texte">
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2) Inactivation of the enzymes for the vector
+
<b>2) Inactivation of the enzymes for the vector</b>
<br>There are two ways to inactivate the enzymes :
<br>There are two ways to inactivate the enzymes :
<br>- Use of DNA Clean up kit for the DNA fragment above 200 pb
<br>- Use of DNA Clean up kit for the DNA fragment above 200 pb
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<p class="title1 " id="select5">Checking of the genetic constructions  </p>
<p class="title1 " id="select5">Checking of the genetic constructions  </p>
 +
<p class="title2">1) Colony PCR</p>
<p class="texte">
<p class="texte">
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1) Colony PCR
+
- Add 0.5µL of plasmid + 25µL of DreamTAQ MasterMix + 2µL of each 10µM primer (VR and VF2) + H<sub>2</sub>0 qsp 25µL and take a colony.
-
<br/>
+
-
- Add 0.5µL of plasmid + 25µL of DreamTAQ MasterMix + 2µL of each 10µM primer (VR and VF2) + H20 qsp 25µL and take a colony.
+
<br/>
<br/>
- Look for the number of necessary cycles and the proper temperature thanks to AmplifX or Serial Cloner 2.1 softwares.
- Look for the number of necessary cycles and the proper temperature thanks to AmplifX or Serial Cloner 2.1 softwares.
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<br/>- (94°C 45sec  ; 55°C 45 sec ; 72°C 1min/kb ) *  25 cycles  
<br/>- (94°C 45sec  ; 55°C 45 sec ; 72°C 1min/kb ) *  25 cycles  
<br/>- 72°C 5min
<br/>- 72°C 5min
-
<br/>- Then 4°C
+
<br/>- Then 4°C</p>
-
<br/>
+
 +
<p class="title2">2) Analytic digestion</p>
<p class="texte">
<p class="texte">
-
2) Analytic digestion
 
-
<br/>
 
- Put a colony in 5mL of LB selective medium and wait for 6 hours
- Put a colony in 5mL of LB selective medium and wait for 6 hours
<br/>
<br/>
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- Mix 2µL of plasmid + 2µL of Fast Digest Green Buffer + 1µL of each enzyme +  Milli-Q water qsp 20µL
- Mix 2µL of plasmid + 2µL of Fast Digest Green Buffer + 1µL of each enzyme +  Milli-Q water qsp 20µL
<br/>
<br/>
-
- Wait 15 minutes at 37°C and put the mix on a 1% or 2% gel for 30 minutes at 100V.
+
- Wait 15 minutes at 37°C and put the mix on a 1% or 2% gel for 30 minutes at 100V.</p>
-
<br/>
+
-
<p class="texte">
+
<p class="title2">3) Sequencing</p>
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<br/>3) Sequencing
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<p class="texte"><br/>The sequencing of the genetic constructions was performed by Eurofins Genomics Company by mixing 15µL of pure plasmid solution with 2µL of one primer.</p>
-
<br/>The sequencing of the genetic constructions was performed by Eurofins Genomics Company by mixing 15µL of pure plasmid solution with 2µL of one primer.
+
<p class="title1" id="select6"> <I>B. subtilis</I> transformation</p>
<p class="title1" id="select6"> <I>B. subtilis</I> transformation</p>
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<p class="texte">
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<p class="texte"><b>Strain:</b> <I>Bacillus subtilis</I> 168.  
-
<br/>Strain: <I>Bacillus subtilis</I> 168.  
+
<br/><b>Plasmid:</b> pSBBS4S given by the Munich University iGEM Team. This plasmid is replicative in <I>E. coli</I> and integrative in <I>Bacillus subtilis</I>.</p>
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<br/>Plasmid : pSBBS4S given by the Munich University iGEM Team. l’équipe iGEM de l’université de Munich. This plasmid is replicative in <I>E. coli</I> and integrative in <I>Bacillus subtilis</I>.
+
<p class="texte">
<p class="texte">
<B> Day 0 </B>
<B> Day 0 </B>
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<br/>- Streak out the Bacillus strain and plate this on an LB agar plate overnight at 37°C
+
<br/>- Streak out the <i>Bacillus</i> strain and plate this on an LB agar plate overnight at 37°C</p>
<p class="texte"><B> Day 1 </B>
<p class="texte"><B> Day 1 </B>
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- Grow the cells at 37°C for an additional 2 hours
- Grow the cells at 37°C for an additional 2 hours
<br/>
<br/>
-
- Spread the complete 400 µl reaction mix on selective antibiotic plates, and incubate at 37°C overnight  
+
- Spread the complete 400 µl reaction mix on selective antibiotic plates (100µl per plate), and incubate at 37°C overnight  
-
<br/>
+
<br/></p>
-
<p class="texte">
+
<p class="texte"><b> Preparation of solutions </b>
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<b> Preparation of solutions </b>
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<I> <br> 300 mM Tri-Na Citrate:</I>
<I> <br> 300 mM Tri-Na Citrate:</I>
<br>- 0.88 g Tri-Na Citrate
<br>- 0.88 g Tri-Na Citrate
<br>- 10mL MQ water
<br>- 10mL MQ water
-
<p class="texte">
+
<br><br><I>Ferric NH4 citrate:</I>
-
<I> <br> Ferric NH4 citrate:</I>
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<br>- 0.22g Ferric NH4
<br>- 0.22g Ferric NH4
<br>- 10mL MQ water
<br>- 10mL MQ water
-
<p class="texte">
+
<br><br><I>10x Competence Medium </I>
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<I> <br> 10x Competence Medium </I>
+
<br> For 10mL:
<br> For 10mL:
<br>- 1.40g K2HPO4
<br>- 1.40g K2HPO4
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<br>- 0.2 g Potassium glutamate
<br>- 0.2 g Potassium glutamate
<br>The complete mixture should be dissolved in 10 ml. First add 5 ml milliQ water and mix. When everything is dissolved add MQ water till 10 ml. Filter sterilize the complete mixture and store at -20°C.
<br>The complete mixture should be dissolved in 10 ml. First add 5 ml milliQ water and mix. When everything is dissolved add MQ water till 10 ml. Filter sterilize the complete mixture and store at -20°C.
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<br><br><I>1x Competence Medium </I>
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<p class="texte">
+
-
<I> <br> 1x Competence Medium </I>
+
<br>- 1.8 mL MQ water
<br>- 1.8 mL MQ water
<br>- 200 µL 10x Competence Medium solution (previously filter sterilized)
<br>- 200 µL 10x Competence Medium solution (previously filter sterilized)

Revision as of 18:37, 16 October 2014