Difference between revisions of "Team:Aix-Marseille/Results"

(Proof of swimming recovery)
(Improvement of FliC E. coli BBa_K342000)
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In a second time, we want to finish the insertion of the restriction site to allow the cassette insertion ( peptide absorbing specifically precious metal) and test their affinity.  
 
In a second time, we want to finish the insertion of the restriction site to allow the cassette insertion ( peptide absorbing specifically precious metal) and test their affinity.  
  
===Improvement of FliC <i>E. coli</i> BBa_K342000===
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===Improvement of FliC <i>E. coli</i> [http://parts.igem.org/Part:BBa_K1463604 BBa_K1463604]===
  
This biobrick has been improoved from a previous one designed by Glasgow 2014 team. Please find the link of this biobrick below :
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This biobrick is an improvement on the biobrick designed by the Glasgow 2014 team.  
http://parts.igem.org/Part:BBa_K1463601
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[http://parts.igem.org/Part:BBa_K1463604 K1463604]
  
Instead of promotors Bba_J23106 and Bba_J23116, we used strong promoter, strong RBS combination for high expression levels of the flagellin. By the combination of Bba_K880005 and Bba_K1951005, we made a high flagellin expression vector able to recover swimming.
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The improvement of this part is multiple.
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* First there is no mutation in the promotor or RBS of our part so the flagellin is well expressed and functional. Unfortunately when the Glasgow team trie to make this part they picked up a mutation in the promotor.
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* Second the sequence that we have used it a synthetic gene with codon optimisation, designed specifically for high level expression in <i>E.coli</i>. Thus as an expression part is improved over the initial design.
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* Third in the functional swimming assay, we see evidence for improved swimming (denser halo), in cells expressing our biobrick, a phenotype not observed by the Glasgow team in 2014.
  
 
==Project achievement in a table==
 
==Project achievement in a table==

Revision as of 21:16, 18 October 2016