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<body> | <body> | ||
+ | |||
+ | <div> | ||
+ | <h2><B>Microbiology Notebook</B></h2> | ||
+ | </div> | ||
+ | |||
+ | <div id="home"> | ||
+ | <center></a><a href="https://2016.igem.org/Team:Pasteur_Paris/Microbiology"><img src="https://static.igem.org/mediawiki/2016/5/5a/Labwork_pasteur.png" width="40%" alt=""/></img></a></center> | ||
+ | </div> | ||
<div id="week10"> | <div id="week10"> | ||
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<a href="#exp2"><h4> 151. Digestion of B2, E1 and C2 from the 4<sup>th</sup> of August </h4></a><br/> | <a href="#exp2"><h4> 151. Digestion of B2, E1 and C2 from the 4<sup>th</sup> of August </h4></a><br/> | ||
<a href="#exp3"><h4> 152. Electrophoresis with the results of digestion </h4></a><br/> | <a href="#exp3"><h4> 152. Electrophoresis with the results of digestion </h4></a><br/> | ||
− | <a href="#exp4"><h4> 153. PCR of inserts A1 | + | <a href="#exp4"><h4> 153. PCR of inserts A1/A2/D1/D2 </h4></a><br/> |
− | <a href="#exp5"><h4> 154. Gel extraction of A1 | + | <a href="#exp5"><h4> 154. Gel extraction of A1/A2/D1/D2 </h4></a><br/> |
<a href="#exp6"><h4> 155. Gel extraction of B2, E1 and E2 </h4></a><br/> | <a href="#exp6"><h4> 155. Gel extraction of B2, E1 and E2 </h4></a><br/> | ||
− | <a href="#exp7"><h4> 156. Resuspension of inserts B2 | + | <a href="#exp7"><h4> 156. Resuspension of inserts B2/E1/E2 </h4></a><br/> |
</p> | </p> | ||
<p><h3><B>August 9, 2016:</B></h3></p> | <p><h3><B>August 9, 2016:</B></h3></p> | ||
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1. Realize a Mastermix and store it on ice : <br /> | 1. Realize a Mastermix and store it on ice : <br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 113</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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<h6><U>Results :</U></h6><br /><br /> | <h6><U>Results :</U></h6><br /><br /> | ||
<center><img src = "https://static.igem.org/mediawiki/2016/c/cf/Week_10_152Electrophoresis_with_the_results_of_digestion.jpg"; alt "Gel of the results of digestion"/> | <center><img src = "https://static.igem.org/mediawiki/2016/c/cf/Week_10_152Electrophoresis_with_the_results_of_digestion.jpg"; alt "Gel of the results of digestion"/> | ||
− | <i><p> <U>Figure | + | <i><p> <U>Figure 18 :</U> Gel of the results of digestion </i></p></center><br /> |
<br /><br /><br /> | <br /><br /><br /> | ||
</p> | </p> | ||
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1. Prepare the following tubes :<br /> | 1. Prepare the following tubes :<br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 114</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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3. Add 1 µl of DNA following the number of tubes : <br /><br /> | 3. Add 1 µl of DNA following the number of tubes : <br /><br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 115</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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<h6><U>Results :</U></h6><br /><br /> | <h6><U>Results :</U></h6><br /><br /> | ||
<center><img src = "https://static.igem.org/mediawiki/2016/b/bb/Week_10_154Gel_extraction_of_A1-A2-D1-D2.jpg"; alt "Extraction gel of A1-A2-D1-D2"/> | <center><img src = "https://static.igem.org/mediawiki/2016/b/bb/Week_10_154Gel_extraction_of_A1-A2-D1-D2.jpg"; alt "Extraction gel of A1-A2-D1-D2"/> | ||
− | <i><p> <U>Figure | + | <i><p> <U>Figure 19 :</U> Extraction gel of A1-A2-D1-D2 </p></i></center> |
<br /><br /> <br /> | <br /><br /> <br /> | ||
</p> | </p> | ||
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Follow the Qiagen Extraction gel kit steps with :<br /><br /> | Follow the Qiagen Extraction gel kit steps with :<br /><br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 116</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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1. Use 1/10 volume of NaAc and 2.5 colume of ethanol for each insert : <br /><br /> | 1. Use 1/10 volume of NaAc and 2.5 colume of ethanol for each insert : <br /><br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 117</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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Use the following volumes : <br /> | Use the following volumes : <br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 118</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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2. Digest the plasmid with the following volumes for each sample : <br /> | 2. Digest the plasmid with the following volumes for each sample : <br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 119</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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<h6><U>Results :</U></h6><br /><br /> | <h6><U>Results :</U></h6><br /><br /> | ||
<center><img src = "https://static.igem.org/mediawiki/2016/a/ad/Week_10_161Electrophoresis_of_the_PCR_done_on_the_8th_of_August_with_A1-A2-D1-D2.jpg" ; alt "Electrophoresis gel of the PCR"/> | <center><img src = "https://static.igem.org/mediawiki/2016/a/ad/Week_10_161Electrophoresis_of_the_PCR_done_on_the_8th_of_August_with_A1-A2-D1-D2.jpg" ; alt "Electrophoresis gel of the PCR"/> | ||
− | <i><p> <U>Figure | + | <i><p> <U>Figure 20 :</U> Electrophoresis gel of the PCR</p></i></center><br /> |
The PCR works properly since we noticed significant bands at the expected level.<br /> | The PCR works properly since we noticed significant bands at the expected level.<br /> | ||
<br /><br /><br /> | <br /><br /><br /> | ||
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1. Realize a master mix with : <br /><br /> | 1. Realize a master mix with : <br /><br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 120</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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1. Put all the following reactants in a 1.5 ml Eppendorf and let digest one hour at 37°C : <br /> | 1. Put all the following reactants in a 1.5 ml Eppendorf and let digest one hour at 37°C : <br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 121</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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<p> | <p> | ||
− | <h6><U> Aim:</U> Have bacteria with the right plasmid to produce our protein. <br/> | + | <h6><U> Aim :</U></h6> Have bacteria with the right plasmid to produce our protein. <br /> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br/><br/> | + | <h6><U> Protocol :</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br /><br /> |
− | <U>What we did in the lab:</U><br/> | + | <h6><U>What we did in the lab:</U></h6><br /> |
− | <U>Materials:</U>< | + | <h6><U>Materials:</U></h6> |
− | • Digested B1 and C2 <br/> | + | • Digested B1 and C2 <br /> |
− | • BL21DE3 competent cells<br/> | + | • BL21DE3 competent cells<br /> |
− | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br/> | + | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br /> |
− | • Shaking incubator (INFORS HT)<br/> | + | • Shaking incubator (INFORS HT)<br /> |
− | • SOC <br/> | + | • SOC <br /> |
− | <U>Method:</U></ | + | <h6><U>Method:</U></h6> |
− | 1. Take 3 samples of C2 v2 (10, 13 and 16) and 2 samples of B1 v2 (6 and 8).<br/> | + | 1. Take 3 samples of C2 v2 (10, 13 and 16) and 2 samples of B1 v2 (6 and 8).<br /> |
− | 2. Put 1 &# | + | 2. Put 1 µl of DNA in 99 µl of H<sub>2</sub>O. Then, put 1 µl of DNA (B1 v2 or C2 v2) in 50 µl of BL21DE3 competent cells.<br /> |
− | 3. Put the samples 30 minutes on ice and then 40 seconds at | + | 3. Put the samples 30 minutes on ice and then 40 seconds at 42°C.<br /> |
− | 4. Put the samples 3 minutes on ice. <br/> | + | 4. Put the samples 3 minutes on ice. <br /> |
− | 5. Add 150 &# | + | 5. Add 150 µl of SOC and let incubate 30 minutes at 37°C and 150 rpm.<br /> |
− | 6. Spread the mix on a petri dish with LB and carbenicillin.<br/> | + | 6. Spread the mix on a petri dish with LB and carbenicillin.<br /> |
− | 7. Let incubate overnight at | + | 7. Let incubate overnight at 37°C and 150 rpm.<br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
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<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Have the concentration of digested pET 43.1 | + | <p> |
− | <U>Results</U>< | + | <h6><U> Aim:</U></h6> Have the concentration of digested pET 43.1(a+) <br /> |
− | <br/><br/><br/> | + | <h6><U>Results</U></h6> Measure the concentration of digested pET 43.1(a+) with a Nanodrop. For the first tube, we find a concentration of 6.8 ng/µl in 46 µl. For the second tube, we find a concentration of 8.8 ng/µl in 46 µl. Then, store the samples at -20°C. <br /> |
+ | <br /><br /><br /> | ||
</p> | </p> | ||
</figcaption> | </figcaption> | ||
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<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Transform C2 v2 and B1 v2 in pET43.1a(+) and DHα . <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim:</U></h6> Transform C2 v2 and B1 v2 in pET43.1a(+) and DHα . <br /> |
− | <U>Results</U>< | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br /><br /> |
− | For B1 v2 and C2 v2 in pET43.1(a+), transformations were successful.<br/> | + | <h6><U>Results</U></h6> For B2 (4, 7, 9), E1 (1, 2) and E2 (2, 3, 4, 5, 6, 7) we see small colonies so we let and 25 µl of carbenicillin.<br /> |
− | For A1, A2 and D1, D2 there were too many bacteria growing so we took a colony, diluted it in LB and then spread it on petri dish with LB, Xgal and carbenicillin. | + | For B1 v2 and C2 v2 in pET43.1(a+), transformations were successful.<br /> |
− | <br/><br/><br/> | + | For A1, A2 and D1, D2 there were too many bacteria growing so we took a colony, diluted it in LB and then spread it on petri dish with LB, Xgal and carbenicillin. <br /> |
+ | <br /><br /><br /> | ||
</p> | </p> | ||
</figcaption> | </figcaption> | ||
</figure> | </figure> | ||
</div> | </div> | ||
− | |||
Line 1,379: | Line 1,388: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> To produce proteins. <br/> | + | <p> |
− | <U>What we did in the lab:</U><br/> | + | <h6><U> Aim:</U></h6> To produce proteins. <br /> |
− | <U>Materials:</U>< | + | <h6><U>What we did in the lab:</U></h6><br /> |
− | • Spectrophotometer Ultrospec 3100<br/> | + | <h6><U>Materials:</U></h6> |
+ | • Spectrophotometer Ultrospec 3100<br /> | ||
• iPTG at 0.5 M | • iPTG at 0.5 M | ||
− | br/><br/> | + | <br /><br /> |
− | <U>Method:</U></ | + | <h6><U>Method:</U></h6> |
− | 1. Make two measurements separated of 30 minutes : | + | 1. Make two measurements separated of 30 minutes : <br /> |
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 122</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
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<th> 6 </th> | <th> 6 </th> | ||
<th> Time of addition of iPTG </th> | <th> Time of addition of iPTG </th> | ||
− | <th> Concentration (ng&# | + | <th> Concentration (ng/µl)</th> |
</tr> | </tr> | ||
</thead> | </thead> | ||
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</table> | </table> | ||
<br/> | <br/> | ||
− | 2. When the OD<sub>600 nm</sub> reached 0.7 keep the last measurement and centrifuge for 3 minutes at 8000 g. <br/> | + | 2. When the OD<sub>600 nm</sub> reached 0.7 keep the last measurement and centrifuge for 3 minutes at 8000 g. <br /> |
− | 3. Throw away the supernatant and store at | + | 3. Throw away the supernatant and store at -20°C. <br /> |
− | 4. Add iPTG to reach 0.3 mM. <br/> | + | 4. Add iPTG to reach 0.3 mM. <br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
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<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Make the future ligation easier. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/c/c0/T--Pasteur_Paris--dephosphorylation_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim :</U></h6> Make the future ligation easier. <br /> |
− | <U>What we did in the lab:</U><br/> | + | <h6><U> Protocol :</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/c/c0/T--Pasteur_Paris--dephosphorylation_protocol.pdf">link</a><br /><br /> |
− | <U>Materials:</U>< | + | <h6><U>What we did in the lab :</U></h6><br /> |
− | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br/> | + | <h6><U>Materials :</U></h6> |
− | • rSAP <br/> | + | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br /> |
− | • CutSmart buffer<br/> | + | • rSAP <br /> |
− | • 1.5 ml Eppendorfs <br/> | + | • CutSmart buffer<br /> |
− | • Distilled water <br/> | + | • 1.5 ml Eppendorfs <br /> |
− | • Shaking incubator (INFORS HT)<br/><br/>< | + | • Distilled water <br /> |
− | <U>Method</U>< | + | • Shaking incubator (INFORS HT)<br /><br /> |
− | 1. Start with tube 2 (8.6 ng&# | + | <h6><U>Method :</U></h6> |
+ | 1. Start with tube 2 (8.6 ng/µl in 46 µl) and use the following mix : <br /> | ||
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 123</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
<th> </th> | <th> </th> | ||
− | <th> Volumes ( &# | + | <th> Volumes ( µl) </th> |
</tr> | </tr> | ||
</thead> | </thead> | ||
Line 1,533: | Line 1,544: | ||
</table> | </table> | ||
<br/> | <br/> | ||
− | 2. Let incubate 30 minutes at | + | 2. Let incubate 30 minutes at 37°C then 5 minutes at 65°C. <br /> |
− | 3. Do the same for tube 1. | + | 3. Do the same for tube 1. <br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,549: | Line 1,560: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Get back the DNA. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim :</U></h6> Get back the DNA. <br /> |
− | <U> What we did in the lab </U>< | + | <h6><U> Protocol :</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a><br /><br /> |
− | < | + | <h6><U> What we did in the lab </U></h6><br /> |
− | <U>Materials:</U>< | + | <h6><U>Materials :</U></h6> |
− | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br/> | + | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br /> |
− | • LB medium <br/> | + | • LB medium <br /> |
− | • Carbenicillin at 50 mg | + | • Carbenicillin at 50 mg/ml <br /> |
− | • B1 | + | • B1/E1/E2 in TOPO <br /><br /> |
− | <U>Method</U>< | + | <h6><U>Method :</U></h6> |
− | We do 31 precultures with a mix with 1 ml of LB and 1 &# | + | We do 31 precultures with a mix with 1 ml of LB and 1 µl of carbenicillin to have :<br /> |
− |   3 samples of E1 <br/> | + |   3 samples of E1 <br /> |
− |   14 samples of B2 <br/> | + |   14 samples of B2 <br /> |
− |   14 samples of E2 | + |   14 samples of E2 <br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,577: | Line 1,588: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Send our insert for sequencing as the transformations in BL21DE3. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br/ | + | <h6><U> Aim :</U></h6> Send our insert for sequencing as the transformations in BL21DE3. <br /> |
− | + | <h6><U> Protocol :</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/c/ca/T--Pasteur_Paris--Transformation_protocol.pdf">link</a><br /><br /> | |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,594: | Line 1,605: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Have precultures to redo the cultures in 4 x 1 l of LB as they grow well. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a><br/ | + | <h6><U> Aim:</U></h6> Have precultures to redo the cultures in 4 x 1 l of LB as they grow well. <br /> |
− | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a><br /><br /> | |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,610: | Line 1,621: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Increase the quantity of plasmid for the next ligation. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a><br/ | + | <h6><U> Aim:</U></h6> Increase the quantity of plasmid for the next ligation. <br /> |
− | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a><br /><br /> | |
<br/><br/><br/> | <br/><br/><br/> | ||
</p> | </p> | ||
Line 1,626: | Line 1,637: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Increase the quantity of DNA. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a><br/ | + | <h6><U> Aim:</U></h6> Increase the quantity of DNA. <br /> |
− | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a><br /><br /> | |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,642: | Line 1,653: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Check if the colonies we took contain the insert. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim:</U></h6> Check if the colonies we took contain the insert. <br /> |
− | <U> What we did in the lab </U>< | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a><br /><br /> |
− | < | + | <h6><U> What we did in the lab </U></h6><br /> |
− | <U> Materials </U>< | + | <h6><U> Materials </U></h6> |
− | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br/> | + | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br /> |
− | • Digestion enzyme Xba I and Hind III <br/> | + | • Digestion enzyme Xba I and Hind III <br /> |
− | • Digestion buffer 2.1 <br/> | + | • Digestion buffer 2.1 <br /> |
− | • 1.5 ml Eppendorfs <br/> | + | • 1.5 ml Eppendorfs <br /> |
− | • Distilled water <br/> | + | • Distilled water <br /> |
− | • Shaking incubator (INFORS HT)<br/> | + | • Shaking incubator (INFORS HT)<br /> |
− | • Inserts B2 | + | • Inserts B2/E1/E2 <br/><br /> |
− | <U> Method </U>< | + | <h6><U> Method </U></h6> |
− | 1. In a 1.5 ml Eppendorf, put : <br/> | + | 1. In a 1.5 ml Eppendorf, put : <br /> |
<table> | <table> | ||
− | <caption align="bottom" align="center">Table | + | <caption align="bottom" align="center"><i><p> <U>Table 124</U></p></i></caption> |
<thead> | <thead> | ||
<tr> | <tr> | ||
<th> </th> | <th> </th> | ||
− | <th> Volumes (&# | + | <th> Volumes (µl) </th> |
</tr> | </tr> | ||
</thead> | </thead> | ||
Line 1,691: | Line 1,702: | ||
</tbody> | </tbody> | ||
</table> | </table> | ||
− | <br/> | + | <br /> |
− | 2. Let incubate one hour at | + | 2. Let incubate one hour at 37°C , then 5 minutes at -20°C. <br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,707: | Line 1,718: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Produce the protein in higher quantity. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/a4/T--Pasteur_Paris--Protein_induction_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim:</U></h6> Produce the protein in higher quantity. <br /> |
− | <U> What we did in the lab </U><br/> | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/a/a4/T--Pasteur_Paris--Protein_induction_protocol.pdf">link</a><br /><br /> |
− | <U> Materials </U>< | + | <h6><U> What we did in the lab </U></h6><br /> |
− | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br/> | + | <h6><U> Materials </U></h6> |
− | • iPTG <br/> | + | • Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>) <br /> |
− | • Carbenicillin at 50 mg | + | • iPTG <br /> |
− | <br/><br/> | + | • Carbenicillin at 50 mg/ml |
− | <U> Method </U>< | + | <br /><br /> |
− | 1. In a 2 l Erlenmeyer, put 1 l of LB and 1 ml of carbenicillin and incubate at | + | <h6><U> Method </U></h6> |
− | 2. For each preculture of 25 ml, put it in a 50 ml Falcon, centrifuge 5 minutes at 3500 rpm, throw away the supernatent and resuspend the pellet in 5 ml of clean LB.<br/> | + | 1. In a 2 l Erlenmeyer, put 1 l of LB and 1 ml of carbenicillin and incubate at 37°C and 150 rpm to warm the liquid.<br /> |
− | 3.Centrifuge 5 minutes at 3500 rpm, throw away the supernatent and resuspend the pellet in 20 ml of clean LB.<br/> | + | 2. For each preculture of 25 ml, put it in a 50 ml Falcon, centrifuge 5 minutes at 3500 rpm, throw away the supernatent and resuspend the pellet in 5 ml of clean LB.<br /> |
− | 4. In each 2 l erlenmeyer, add 5 ml of our preculture : 4 erlenmeyer for C2 and 4 for B1. <br/> | + | 3.Centrifuge 5 minutes at 3500 rpm, throw away the supernatent and resuspend the pellet in 20 ml of clean LB.<br /> |
− | 5. Let incubate at 37 °C ann 150 rpm and measure the DO. <br/> | + | 4. In each 2 l erlenmeyer, add 5 ml of our preculture : 4 erlenmeyer for C2 and 4 for B1. <br /> |
− | 6. Once the DO reaches 0.7, add 1 ml of iPTG.<br/> | + | 5. Let incubate at 37 °C ann 150 rpm and measure the DO. <br /> |
− | 7. Let incubate for 3 hours. <br/> | + | 6. Once the DO reaches 0.7, add 1 ml of iPTG.<br /> |
− | 8. Centrifuge the cultures. <br/> | + | 7. Let incubate for 3 hours. <br /> |
− | 9. Resuspend the pellet in 10 ml of lysis buffer (See protein purification protocol) in a 50 ml Falcon of known weight.<br/> | + | 8. Centrifuge the cultures. <br /> |
− | 10. Store at | + | 9. Resuspend the pellet in 10 ml of lysis buffer (See protein purification protocol) in a 50 ml Falcon of known weight.<br /> |
− | <br/><br/><br/> | + | 10. Store at -20°C. <br /> |
+ | <br /><br /><br /> | ||
</p> | </p> | ||
</figcaption> | </figcaption> | ||
Line 1,739: | Line 1,751: | ||
<figcaption> | <figcaption> | ||
− | <p><U> Aim:</U> Check if the digestion works. <br/> | + | <p> |
− | <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/6/60/T--Pasteur_Paris--Gel_electrophoresis_protocol.pdf">link</a><br/><br/> | + | <h6><U> Aim:</U></h6> Check if the digestion works. <br /> |
− | <U> What we did in the lab </U><br/> | + | <h6><U> Protocol:</U></h6> follow in this <a href="https://static.igem.org/mediawiki/2016/6/60/T--Pasteur_Paris--Gel_electrophoresis_protocol.pdf">link</a><br /><br /> |
− | <U> Materials </U>< | + | <h6><U> What we did in the lab </U></h6><br /> |
− | • Agarose <br/> | + | <h6><U> Materials </U></h6> |
− | • Qiagen kit <br/> | + | • Agarose <br /> |
− | • Nanodrop <br/> | + | • Qiagen kit <br /> |
− | • Electrophoresis chamber <br/> | + | • Nanodrop <br /> |
+ | • Electrophoresis chamber <br /> | ||
• Loading buffer 6X | • Loading buffer 6X | ||
− | <br/><br/> | + | <br /><br /> |
− | <U> Method </U>< | + | <h6><U> Method </U></h6> |
− | 1. Add 10 &# | + | 1. Add 10 µl of loading buffer 6X to reach 50 µl for each sample.<br /> |
− | 2. Do an electrophoresis and extract the bands of the palsmid digested. We obtaines two tubes : <br/> | + | 2. Do an electrophoresis and extract the bands of the palsmid digested. We obtaines two tubes : <br /> |
− |   Tube1 : m1 = 1.276 − 0.9964 = 131.2 mg <br/> | + |   Tube1 : m1 = 1.276 − 0.9964 = 131.2 mg <br /> |
− |   Tube2 : m2 = 1.1524 − 0.9994 = 153.0 mg <br/> | + |   Tube2 : m2 = 1.1524 − 0.9994 = 153.0 mg <br /> |
− | 3. Follow the Qiagen kit steps for a final volum of 50 &# | + | 3. Follow the Qiagen kit steps for a final volum of 50 µl.<br /> |
− | 4. Measure the concentration with the Nanodrop to see the results.<br/> | + | 4. Measure the concentration with the Nanodrop to see the results.<br /> |
− | 5. Store at | + | 5. Store at -20°C.<br /><br /> |
− | <U>Results</U>< | + | <h6><U>Results</U></h6> |
− | Tube 1 : 20 .2 ng&# | + | Tube 1 : 20 .2 ng/µl<br /> |
− | Tube 2 : 24.8 ng&# | + | Tube 2 : 24.8 ng/µl <br /> |
− | <br/><br/><br/> | + | <br /><br /><br /> |
</p> | </p> | ||
</figcaption> | </figcaption> |