Team:Yale/Project MAGE

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=== Next steps ===
=== Next steps ===
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*The next step is to grow up these cultures (we sorted our 1,000 cells each time to start a culture).
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*The next step is to grow up these cultures (we sorted out 1,000 cells from each culture to start a culture).
*These cells will be tested on the plate reader compared to the wild type EcNR2, as well as the wild type EcNR2 with our plasmid.  The  MAGEd and FACS sorted cells should show an increased levels of fluorescence, due to increased PLA production.  With only 1 MAGE cycles we were able generate a twofold increase, so in theory with an additional 5 MAGE cycles this increase will be even more drastic.
*These cells will be tested on the plate reader compared to the wild type EcNR2, as well as the wild type EcNR2 with our plasmid.  The  MAGEd and FACS sorted cells should show an increased levels of fluorescence, due to increased PLA production.  With only 1 MAGE cycles we were able generate a twofold increase, so in theory with an additional 5 MAGE cycles this increase will be even more drastic.
*This experiment will be done within the next week and the results will be presented at the regional competition
*This experiment will be done within the next week and the results will be presented at the regional competition

Revision as of 00:14, 28 September 2013

Contents

MAGE Targets

  • The first step in applying MAGE is finding MAGE targets. This involved reading numerous scientific papers to learn as much as possible about the heterologous enzymes, and the pathway that was being used to create the PLA

Enzyme Targets

  • Sadly there was no crystal structure of either enzyme we could use to locate the sites to introduce mutations
    • However, we used the literature available to locate spots where we would want to introduce mutations


Propionate CoA-transferase

  • According to Selmer et al. 2002, there is a catalytic glutamate found in all CoA-transferases
  • Using alignment tools along with the crystal structure of YdiF CoA transferase (That shares 45% sequence identity with the Propionate CoA-transferase) we were able to locate the catalytic glutamate in our enzyme
  • Also, we were able to locate the oxyanion hole of the enzyme
  • We also targeted the regions mentioned in the Lee papers
PCTmagetargets.jpg


P. resinovorans PHA synthases

  • From Yang et al. 2011 we knew there were 4 targets for mutation that affected the efficiency of this enzyme (E130, S325, S477, and Q481)
  • After some more reading we found three amino acids that were putative catalytic residues (C296, D451, and H479)
  • This gave the impression of one hotspot area (amino acids 477-481) so an oligo was designed to target the enzymes in between (AA478 and AA480)
PHAMAGE.JPG

Pathway Engineering

  • We wanted to divert resources toward our desired pathway
    • This mainly consisted of increasing the production of lactate
    • In order to better understand the pathway we were tampering with we created this metabolic engineering graphic (using the sources listed at the bottom of this page)

Metabolic Engineering Graphic.png

Enzyme KOs

  • This led us to find 8 targets for Knockouts (enzymes which would divert resources from our desired pathway)
    • These include adhE, ackA, pfl(A,B), frd(A,B,C,D, ppc, atoB, pta, eutD
    • Oligos were designed to introduce two nonsence mutation near the begining of these ezymes, so they would not be expressed
    • Using Flux Balance Analysis (instructions here) we were able to determine that none of these enzymes would cause a fitness hit except ppc
FBAKO.JPG




RBS Tuning

  • Using the pathway diagram shown above we found 20 enzymes that could be potential targets for mutation
    • Using the same approach taken in MAGE paper (Wang et al. 2009), we designed oligos that target the RBS of each enzyme, and made the oligos degenerate with the following sequence DDRRRRRDDDD (-4 through -14 positions from the start codon)
    • This would alter the RBS to adjust transcription and thus allow some cells to have higher expression and some cells have lower expression
    • Using FACS we would be able to sort through the cells and determine which cells have the highest PLA production
    • The figure shows how to design a oligo depending on which strand and which replichore the gene is located.
    • Here is a link to the 20 Enzymes targeted for RBS tuning
    • Here is a link to the sequences of the 28 Oligos for RBS tuning
Mage3.jpg


Results

  • The first time we used FACS to sort the cells, we saw roughly a two fold increase in fluorescence when we tested on the plate reader after only 1 round of MAGE with the KO oligos

FACSsortingBandA.jpg

  • We used this 3 cultures of this FACS sorted strain and ran 5 more MAGE cycles each culture (one culture was MAGEd with the RBS oligos, one with KO, and one with all Oligos)
    • Here are the results of the FACS sorting of these strains
The first sample is the baseline. This is EcNR2 with our plasmid containing both the PCT and PHA gene. This strain was grown overnight with the cells induced and in the presence of Nile red to strain the PLA (this is the same procedure for all later strains as well). The gate (labeled P2) was chosen to select those with the highest levels of fluorescence. Due to the abnormally high levels of fluorescence in some cells in the baseline, the gate was chosen to include some baseline cells, but only those with very high levels of fluorescence. Baseline both.jpg
The second sample is the KO oligos. This means it had a pool of 11 oligos to knock out 11 enzymes. The enzymes targeted for Knockout were ackA, frdB, frdD pflA, pflB, adhE, frdA, frdC, ATOB, PTA, EUTD. The chart shows that 26 cells within the P2 gate compared to the 15 in the baseline. That means number of cells with high levels of fluorescence nearly doubled. 64-KO knockouts both.jpg
The third sample is the RBS tuning olgios. These are oligos have degenerate RBS site with the following sequence DDRRRRRDDDD (-4 through -14 positions from the start codon). The enzymes targeted for RBS tuning are DHA, ACS, ATOB, EUTD, PTA, MAEA, MAEB, PYKF, ENO, PGM, PGK, GAPA, TPIA, FBAA, FBAB, PFKA, PFKB, GLK, PGL, RPOS. The number of cells within the P2 gate is 65, which is greater than a fourfold increase compared to the baseline. 64-RBS both.jpg
The fourth sample is the all oligs. This is a combination of both the RBS oligos and the KO oligos. This sample has 98 cells within the gate, which is a six and a half fold increase. 66-All both.jpg
Due to the fact the last sample with all the oligos had so many cells within the gate we decided to make a stringent gate. This gate was moved to only select the top 0.1% of the cells. This corresponded to 7/10,000. These cells were collected as well as the cells from the three previous graphs 66-All high both.jpg

Next steps

  • The next step is to grow up these cultures (we sorted out 1,000 cells from each culture to start a culture).
  • These cells will be tested on the plate reader compared to the wild type EcNR2, as well as the wild type EcNR2 with our plasmid. The MAGEd and FACS sorted cells should show an increased levels of fluorescence, due to increased PLA production. With only 1 MAGE cycles we were able generate a twofold increase, so in theory with an additional 5 MAGE cycles this increase will be even more drastic.
  • This experiment will be done within the next week and the results will be presented at the regional competition




List of Papers

Jacob et al. 1997
Matsuzaki et al. 1998
Sawers et al. 1998
Park et al. 2002
Selmer et al. 2002
Takase et al. 2002
Fong et al. 2005
Matsumoto et al. 2005
Rangarajan ES et al. 2005
Matsumoto et al. 2006
Jung et al. 2009
Matsumoto et al. 2009
Juang et al. 2010
Orth et al. 2010
Yang et al. 2011
Kandasamy et al. 2012
Yang et al. 2013

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