Data-processing.

We successfully screened two mutants (I208V & R90A ) with higher enzyme activity by site-directed mutation.
You can find our part pages here:I208V      R90A

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Results of Microbial Consortium

Optimization of Culture Conditions

1. Exploration for an appropriate medium

(1) Co-culture in LB medium

(2) Co-culture in YPD medium

(3) Co-culture in M9 medium

We cultured bacteria as experiments for three days, and checked the bacterial concentration at OD₆₀₀(See Fig.2 in details) and detectd the concentration of TPA by UV at OD₂₄₂(See Fig.3 in details).

After analyzing graphs, easily, we can get a conclution that Rhodococcus jostii RHA1 can degrade TPA particularly well and Pseudomonas putida KT2440 can not degrading TPA. Obviously, Rhodococcus jostii RHA1 and Pseudomonas putida KT2440 can not live with each other in M9 medium because Group R.j + P.p is the same as control regarding concentration of TPA.

(4) Co-culture in W medium

We cultured bacteria as experiments for three days, and checked the bacterial concentration at OD₆₀₀(See Fig.4 in details) and detectd the concentration of TPA by UV at OD₂₄₂(See Fig.5 in details), then, observed some sample with microscope(See Fig.6 in details)

By Fig.4 and Fig.5, we can find that TPA of both Group R.j and Group R.j + P.p was degraded markedly, and degrading quantity of Group R.j + P.p is slightly larger than Group R.j. Then, by Fig.4, Fig.5, Fig.6, Fig.7, Rhodococcus jostii RHA1 and Pseudomonas putida KT2440 can be co-cultured in W medium. Besides, Bacillus stubtilis can grow better in W medium compared with M9 medium.

2. Adjustment of nitrogen source

We choose two groups of experiments to show how to change growing condition of bacterial consortium by adjusting nitrogen source. Cell growth curve and TPA concentrations changes in W2 and W3 medium are shown as Fig.8, Fig.9 and Fig.10, Fig.11, respectively.

By analyzing data we have had, Bacillus stubtilis grow best in W3 medium, and in W2 and W3 medium, group RPB can both degrading TPA well. Because Bacillus stubtilis is main player to secret PETase and MHETase, we decide to add KNO3 to adjust nitrogen source at last.

3. Temperature

We cultured Rhodococcus jostii RHA1, Pseudomonas putida KT2440, Bacillus stubtilis 168 in W9 medium at 30 degrees and 37 degrees respectively. Growing conditions of bacteria the next day are shown as Fig.12.

We found that Bacillus stubtilis grew a little better at 37 degrees, however, Rhodococcus jostii could not grow at 37 degrees. So we finally chose 30 degrees as culture degree of bacterial consortium.

4. Influence of Cl^-

By accident, I found Bacillus stubtilis could not grow well without Cl^-, but Rhodococcus jostii RHA1, Pseudomonas putida KT2440 grew as usual. Therefore, we prepared a series of medium(add NaCl to W medium without NH4Cl ) to explore influence of Cl^-. Growing conditions of Bacillus stubtilis the next day are shown as Fig.13.

(PS: Because W9 medium includes NH4Cl that disrupts our exploration to influence of Cl-, so we replace NH4Cl with (NH4)2SO4 which consists of same concentration of NH4+.)

From Fig.13, we conclude that increasing the concentration of Cl^-can contribute to growth of Bacillus stubtilis, but after exceeding certain concentration, acceleration of Cl^-disappears.

5. Adjustment of carbon source

We added sucrose to improve growing condition of Bacillus stubtilis, then, Cell growth curve and TPA concentrations changes in W9 medium are shown as Fig.14, Fig.15, respectively.

6.Optimum medium

Basing on experiments above, we synthesize some conclusion and design some better media to give bacterial consortium a better surrounding to degrading PET. After processing data, we find W18 medium (without PET films) can make our consortium work better(Fig.16 and Fig.17).

To our delight, in the medium, Bacillus stubtilis can grow better than experiments before and group RPB can degrading TPA more efficiently. Eventually, we succeed in construct a relatively more stable bacterial consortium.

Later, in order to confirm coexist of three bacteria, we firstly observed sample under the microscope(Fig.18 and Fig.19).

Regrettably, results of microscopic examinations can not confirm coexist of three bacteria certainly, therefore, we use 16SrDNA to examine further.

7.results of the first colony-pcr of 16s-rDNA: provident the specificity of the primers

If number 1 had a set of DNA molecules rather than number 2/3, we got the conclusion that the primers—‘RJ-S/A’ could only get the 16s-rDNA gene of Rhodococcus RHA1 rather than ones in Pseudomonas putida KT2440 and Bacillus subtilis 168. Also,DNA molecules in number 5 and 9 could prove the specificity of the primers of other two bacteria.

8.results of the second colony-pcr: provident the possibility of consortium

On six parallel lanes of the gel(number 1,5,9,10,11,12), six set of DNA molecules of known size( 1000bp for number 1 and 10 ; 1500bp for number 5 and 11; 1600bp for number 9 and 12) were run. From the DNA band of number 1,5 and 9，we could analyze that three bacteria growed well in each modified W0 culture medium. From the DNA band of number 10,11 and 12 , we could delightedly prove that three bacteria growed well together in the modified W0 culture medium.

In conclusion, we cultivated consortium of three bacteria in the modified W0 culture medium by the validation of 16s-rDNA.

Modification of Bacillus subtilis

1.the degree of PET degradation in Bacillus subtilis

2.the degree of PNPA degradation——new discovery

We make the first step of PNPA degradation after the success of transport. However, we fail to find the absorption peak of PNP at 400nm in experimental group.At first ,we attribute this result to PNP decomposition(Figure 25).Then, we search on the Internet and find that Bacillus subtilis has the ability to degree PNP.So we cannot use the degree of PNPA degradation to measure enzymatic activity.

Modification ofPseudomonas putida KT2440

Proof of overexpression in P.putida KT2440

After the experiment design was finally confirmed, we started to establish the overexpression vector based on the shuttle plasmid pBBR1MCS-2 as we described on the Experiment Page. The aim of this overexpression vector is to make KT2440 utilize EG more efficient and tend to accumulate PHA in bacterial body.

After plasmid pBBRAA (pBBR linked with AcoA and AceA) was successfully transformed into E.coli, we amplified and extracted it from E.coli to prove that the target genes had been successfully ligated into pBBR. We proved it by PCR of pBBRAA and the result is showed as below.

The PCR’s results confirmed that the target genes were ligated into pBBR, which meant the overexpression was successfully established. Then, we transformed it into P.putida KT2440 by electroporation.However, we met some problem unsolved in the electroporation.So we need some improvement in the future.

We hope that after adding nickel sulfate to the cultures, cyanobacteria could split in a few days, releasing plenty of lipid to feed others as the source of carbon in our mixed bacteria system.

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Results of R-R system

Results of inclusion body based reporting system.

The red fluorescence can be observed by bare eyes. We set up four groups:
A. No E.coli.
B. E.coli with empty plasmid pUC19.
C. E.coli with pUC19+CpxR-RFP.
D. E.coli with pUC19+CpxR-RFP+PETase gene.
The result is as the following picture. (After centrifugation with the speed of 12000rpm for 1min)

We found that the group with part BBa_K339007 and PETase gene showed deepest red in all of the four groups. The group with only part BBa_K339007 also showed a little red, we speculate that this might be caused by the basic expression of some genes in E.coli and some of the expression products formed inclusion bodies. It might also be caused by the basic expression of the RFP gene because the CpxR promoter might also, though not so strongly, start the transcription even without the induction of CpxR protein. The group with empty plasimd did not showed any red color and the group with no E.coli cultured did not have any sediment at the bottom of tube.

2.Results of cell lysis effect of ddpX gene.

We first did a experiment to measure the cell lysis effect of ddpX gene. We simply use the IPTG inducible T7 promoter to regulate the expression of ddpX gene. We totally set four groups:
1. E.coli wildtype.
2. E.coli wildtype added IPTG.
3. E.coli with ddpX gene, no induction.
4. E.coli with ddpX gene, IPTG added as induction.
Then we continuously measure the OD₆₀₀ of the culture medium by 96-well Microplate Reader and draw the OD₆₀₀-culturing time curve by Matlab. The graph is showed below.

From this image, we can see that in the first 5 hours, the OD₆₀₀ of each group is almost the same because of the rich nutrition and the ddpX cannot take effect immidiately. However, after 5 hours, the group with ddpX transformed and IPTG induced showed the fastest decrease among all the groups. This is because of the cell lysis effect of ddpX. Comparing the group with ddpX gene and IPTG inducted with the group with wildtype bacterial and the same amount of IPTG added we can draw the conclusion that the ddpX gene can cause cell lysis significantly. However, the data of another two groups are a little strange. We think it is because of the basic expression of ddpX can partly hydrolyze the peptidoglycan in the cell wall and provide cells with D-Ala as carbon source. This is exactly the physical use the the ddpX gene when the cell is under starvation condition, see more details about this explanation in our experiment page. Therefore the group with ddpX gene but no induction can live longer and better when the nutritions are deficient.

Summary

1.We successfully established a special bacteria consortium-Bacillus stubtilis 168 or DB104, Rhodococcus jostii RHA1 and Pseudomonas putida KT2440 for this enzyme catalysis reaction. We use 16s-rDNA to prove the existence of special bacteria consortium.

2.We optimized culture conditions by changing carbon source, nitrogen source and some ions. After checking the growth situations and conditions of the degrading PET, TPA and EG, we explore a suitable culture condition to co-culture our bacteria consortium.

3.We constructed pHP13-P43-PETase/MHETase plasmid for Bacillus stubtilis 168 or DB104. The recombinant strain had the ability to degree PET. Also, we found PNPA couldn’t characterize of enzyme hydrolysis rate.

4. In order to increase the Pseudomonas putida KT2440’s intake of EG, we found the main influential genes---AceA and AcoA and successfully established an overexpression vector in Pseudomonas putida KT2440, which makes this bacterium can utilize EG more efficiently.

5.We successfully applied and improved the previous part BBa_K339007 designed and constructed by the Group iGEM10_Calgary to construct our inclusion body based reporting system and inclusion body based cell lysis regulation system.

6.The red fluorescence can even be directly observed by bare eyes when we express the PETase gene in E.coli which was transformed into the CpxR-RFP fragment.

7.We measured the cell lysis effect of the novel ddpX gene and combined it with the PETase expression system in E.coli.