Difference between revisions of "Team:Evry/Protocols"

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<br>19 µl colony resuspended Luria Bertoni media in 4 mL of Luria Bertoni media complemented with 4 µl of ampicilin (100 mg/µl) and put to incubate at 37°C overnight.
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19 µl colony resuspended Luria Bertoni media in 4 mL of Luria Bertoni media complemented with 4 µl of ampicilin (100 mg/µl) and put to incubate at 37°C overnight.
 
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<li>1) 5 spleens from C57BL/6 mice were digested in 5 mL of Collagenase/DNase for 45 minutes à 37°C.</li>
 
<li>1) 5 spleens from C57BL/6 mice were digested in 5 mL of Collagenase/DNase for 45 minutes à 37°C.</li>
 
<li>2) The reaction was stopped by 0.6 mL of PBS/EDTA.</li>
 
<li>2) The reaction was stopped by 0.6 mL of PBS/EDTA.</li>
 
<li>3) The organs digested were filtered 70 μ et centrifuged 10 minutes at 1300 rpm.</li>
 
<li>3) The organs digested were filtered 70 μ et centrifuged 10 minutes at 1300 rpm.</li>
 
<li>4) FC receptors were saturated before magnetic separation</li>
 
<li>4) FC receptors were saturated before magnetic separation</li>
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     <li> 1) Dendritics cells or macrophages were seeded at 1.105 cells per well in U-bottom 96-well plates in complete RPMI medium.</li>  
 
     <li> 1) Dendritics cells or macrophages were seeded at 1.105 cells per well in U-bottom 96-well plates in complete RPMI medium.</li>  
 
     <li> 2) Recombinant S. cerevesiae or soluble SIINFEKL protein were added at various concentrations. </li>
 
     <li> 2) Recombinant S. cerevesiae or soluble SIINFEKL protein were added at various concentrations. </li>
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  <li> 4) Plates were washed once with PBS and 􏰁beta-galactosidase activity was assessed by the addition of 120 u􏰃l of lysis buffer (PBS, 9 mM MgCl2, 0.125% NP40 and 0.15 mM chlorophenolred-galactoside (CPRG).</li>
 
  <li> 4) Plates were washed once with PBS and 􏰁beta-galactosidase activity was assessed by the addition of 120 u􏰃l of lysis buffer (PBS, 9 mM MgCl2, 0.125% NP40 and 0.15 mM chlorophenolred-galactoside (CPRG).</li>
 
  <li> 5) After the color shift to red, the absorbance at 570 nm was read on a micro-plate reader.</li>
 
  <li> 5) After the color shift to red, the absorbance at 570 nm was read on a micro-plate reader.</li>
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Acquisition was performed at Genethon, Genpole (Evry) with a flow cytometer.  
 
Acquisition was performed at Genethon, Genpole (Evry) with a flow cytometer.  
<br>For surface display staining with HA-tag-680 label, yeasts were grown at 30°C with 300 r.p.m. agitation in SC-auxotrophic complemented media.  
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<br>- For surface display staining with HA-tag-680 label, yeasts were grown at 30°C with 300 r.p.m. agitation in SC-auxotrophic complemented media.  
<br>When culture reached mid-exponential phase, cells were harvested and fixed with paraformaldehyde with the following protocol : 1 mL sample was cooled to an ice water-bath and centrifuged at 4°, 2000g for 2 min.  
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<br>- When culture reached mid-exponential phase, cells were harvested and fixed with paraformaldehyde with the following protocol : 1 mL sample was cooled to an ice water-bath and centrifuged at 4°, 2000g for 2 min.  
<br>Antibodies were added during 30 minutes, then the cells were washed with PBS. Supernatant was removed and pellet was resuspended in 200 uL of 0.5 % paraformaldehyde. The mix was incubated on ice for 30 minutes and subsequently centrifuged at 4°C, 2000g for 2 minutes.  
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<br>- Antibodies were added during 30 minutes, then the cells were washed with PBS. Supernatant was removed and pellet was resuspended in 200 uL of 0.5 % paraformaldehyde. <br>- The mix was incubated on ice for 30 minutes and subsequently centrifuged at 4°C, 2000g for 2 minutes.  
 
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Revision as of 01:19, 19 September 2015

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