Difference between revisions of "Team:Evry/Project/Biosensor"

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<il><strong>A.</strong> In vitro delivery of granzyme B to colon cancer cells with perforin resulted in caspase 3 activation and features of apoptosis in those cells : chromatin condensation, nucleus fragmentation and internucleosomal DNA fragmentation (8)</il>
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<il><p class="text-justify"><strong>A.</strong> In vitro delivery of granzyme B to colon cancer cells with perforin resulted in caspase 3 activation and features of apoptosis in those cells : chromatin condensation, nucleus fragmentation and internucleosomal DNA fragmentation (8)</p></il>
<il><strong>B.</strong> Recombinant Granzyme B and perforin co-expressed in E. coli induced apoptosis and directly inhibited the growth of human laryngeal cancer Hep-2 cells in vitro (9)</il>
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<il><p class="text-justify"><strong>B.</strong> Recombinant Granzyme B and perforin co-expressed in E. coli induced apoptosis and directly inhibited the growth of human laryngeal cancer Hep-2 cells in vitro (9)</p></il>
 
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<img border="0" class='img-responsive' width="500" src="https://static.igem.org/mediawiki/2015/7/7e/Manquante2.png" alt="" />
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<p class="text-justify"><strong>Figure 3 : Yeast encapsulated secreting perforine and granzyme B upon hypoxia detection</strong></p>
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<p class="text-justify">For optimal conditions of translation, we placed both proteins on the same mRNA under control of the CMV minimal promoter. The Internal Ribosome Entry Site IRES URE2, effective in yeast, was placed ahead of the second protein to ensure two translations on the same mRNA.</p>
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<p class="text-justify">Two different secretion signal, Matalpha leader peptide and BGL2 signal peptide, were fused to each protein to avoid internal recombination during expression.</p>
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<p class="text-justify">Sequencing data showed the correct cloning of all the constructions producing Granzyme B and perforine. In vitro characterization remains to be done with these constructions.</p>
  
  

Revision as of 00:04, 19 September 2015

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