Team:INSA-Lyon/Results
From 2014.igem.org
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<div><h5><p align="center"> <b>Curli formation and adherence properties conferred by the 3 constructs CsgA-WT, CsgA-His1 and CsgA-His2</b></p></h5> | <div><h5><p align="center"> <b>Curli formation and adherence properties conferred by the 3 constructs CsgA-WT, CsgA-His1 and CsgA-His2</b></p></h5> | ||
<p align="justify">5 complementary tests were performed to evaluate the ability of the modified cells to assemble functional curli: 1) determination of the percentage of adherent cells to polystyrene in 24 wells-plates, 2) crystal violet staining of biofilm formed on polystyrene in 24 wells-plates, 3) ability to bind the congo red, 4) biofilm maximum thickness measurement and biovolumes quantification of GFP-tagged biofilm observed with a confocal microscopy and 5) curli structure observation using Transcription Electron Microscopy (MET).</p> | <p align="justify">5 complementary tests were performed to evaluate the ability of the modified cells to assemble functional curli: 1) determination of the percentage of adherent cells to polystyrene in 24 wells-plates, 2) crystal violet staining of biofilm formed on polystyrene in 24 wells-plates, 3) ability to bind the congo red, 4) biofilm maximum thickness measurement and biovolumes quantification of GFP-tagged biofilm observed with a confocal microscopy and 5) curli structure observation using Transcription Electron Microscopy (MET).</p> | ||
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<h6>Adhesion test and curli production</h6> | <h6>Adhesion test and curli production</h6> | ||
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Strains with our parts, the positive and negative control were cultivated in M63 Mannitol at 30°C and 180rpm. After centrifugation, the supernatant was removed and the cell pellet was resuspended in the Congo Red solution, in order to specifically stain the curli. The samples were centrifuged again and the pellets observed (See protocol for more details). <br/> | Strains with our parts, the positive and negative control were cultivated in M63 Mannitol at 30°C and 180rpm. After centrifugation, the supernatant was removed and the cell pellet was resuspended in the Congo Red solution, in order to specifically stain the curli. The samples were centrifuged again and the pellets observed (See protocol for more details). <br/> | ||
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- | Congo Red staining shows that <b>the CsgA with one or two tag from the P70 promoter allows to form curli fiber</b> which are able to bind congo red. <br/></p> | + | Congo Red staining shows that <b>the CsgA with one or two tag from the P70 promoter allows to form curli fiber</b> which are able to bind congo red.<br/></p> |
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<h6>Confocal Laser Scanning Microscopy Analyzes</h6> | <h6>Confocal Laser Scanning Microscopy Analyzes</h6> | ||
<div align="justify"><p><br/>For the Confocal Laser Scanning Microscopy biofilm acquisitions, all the strains were cultivated in 96-wells microplate in M63 Mannitol during 16H at 30°C (<a href="https://static.igem.org/mediawiki/2014/7/7e/Culture_confocal_analyse.pdf">See Protocol for details</a>). See results in <b>Figure 4</b>.</p> | <div align="justify"><p><br/>For the Confocal Laser Scanning Microscopy biofilm acquisitions, all the strains were cultivated in 96-wells microplate in M63 Mannitol during 16H at 30°C (<a href="https://static.igem.org/mediawiki/2014/7/7e/Culture_confocal_analyse.pdf">See Protocol for details</a>). See results in <b>Figure 4</b>.</p> |
Revision as of 19:30, 17 October 2014