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

(Proof of protein production)
(Proof of fonctionnality)
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=== Proof of fonctionnality===
 
=== Proof of fonctionnality===
We investigated if DesA (Lysine decarboxylase) was fonctionnal, by measurement of cadaverine using HPLC with C18 column and proofed our biobrick is a producer of this protein and makes it fonctionnal.
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[[File:T--Aix-Marseille--result5.jpeg|500px|right|thumb|Test of our biobrick proteins production using a SDS page and comassie. - : no induction ; + : induction with 0.02% arabinose at Abs(600nm)=0.4]]
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We investigated if the DesA, DesB, DesC and DesD proteins were well produced by our biobrick using SDS PAGE.  
  
[[File:T--Aix-Marseille--result1.jpeg|770px|center|thumb|<u>On the right</u>, we tested the protein production using a SDS page and comassie in a <i>Escherichia coli</i> Tg1 strain after transformation with Bba_K1951011. On the right column, it has been observed the protein production without induction with 0.02% arabinose. On the left column, protein production was tested after induction. Results showed the production of the 4 proteins DesA, DesB, DesC and DesD, all involved in the desferrioxamine biosynthesis pathway. <u> On the left, </u> we had a look of the cadaverine production by the lysine decarboxylase DesA. Production has been detected by HPLC using C18 column after induction of the strain. <i>Escherichia coli</i> Tg1 strain was used as a wild type. Cadaverine production has been detected in this strain. In a Tg1 cadA mutant, cadaverine was also produced in a least quantity showing that an other pathway is responsible for the production of cadaverine. In the cadA mutant complemented by Bba_K1951004, the amount of cadaverine was recovered and even beyond the wild type production. Moreover, in the cadA mutant complemented by Bba_K1951011, the cadaverine level produced was even over the wild type and complemented Bba_K1951004 production ]]
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To do this we performed SDS PAGE and stained with comassie blue using cells containing this biobrick in plasmid backbone [https://2016.igem.org/Team:Aix-Marseille/Experiments/Protocols Find here the protocol] From an over night starter, cells were diluted and grown from Abs(600nm)=0.2 to Abs(600nm)=1.
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Then 1UOD of cells (1.67ml at 0.6OD) was collected and centrifuged at 5000g for 5min.
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After removal of the supernatant, the cell pellet was resuspended in 50µL SDS-PAGE sample buffer.
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We heated the mix at 95°C during 15min
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[https://2016.igem.org/Team:Aix-Marseille/Experiments/Protocols Find here the protocol]
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The mixture was loaded onto a polyacrylamide gel and migrated during 50min at 180V.
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Staining was done using coomassie blue.
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We compared the production of proteins in different background :
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- <i>E. coli</i> Tg1 strain without any plasmide (negative temoin)
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- <i>E. coli</i> Tg1 strain with pSB1C3 containing the RFP coding sequence (negative temoin)
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- <i>E. coli</i> Tg1 strain complemented with our biobrick Bba_K1951011 before and after induction. (you can observe the production of the 4 proteins on the figure below on the left; right : before induction, left : after induction)
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Results showed the production of the 4 proteins DesA, DesB, DesC and DesD, all involved in the desferrioxamine B biosynthesis pathway.
  
 
===In the futur===  
 
===In the futur===  

Revision as of 21:31, 18 October 2016