Team:Bielefeld-CeBiTec/Results/rMFC/Construction
From 2014.igem.org
Module I - reverse microbial fuel cell (rMFC)
Construction of an electrobiochemical reactor
We planned to design a reactor system that is suitable to investigate the electrochemical behaviour in bioprocesses. That includes the possibility to characterize mediators and different electrode materials on the one hand and the electron uptake into the cells on the other.
During our research we discovered the H-cell reactor that seemed to meet with our needs. (Park et al., 1999)
The advantages of an electrochemical measuring cell with separated compartments are that there is no mixing within the nascent products of electrolysis of the anode- and cathode compartment and the possibility to use different buffers in both compartments.
We approached two different concepts to realize the reactor construction. One of our H-cell reactors was constructed with the possibilities by the glass workshop department of our university. Besides that the technical workshop build the lids from stainless steel. This approach had the advantage that we could influence the design and had to make precise design drawings especially for the connections in the lids.
The second H-cell reactor was a commercially available system by Adams & Chittenden scientific glass. The commercial system had a smaller volume and the benefit of a larger flange diameter. The necessary lids for that system were also custom design by our workshop. In figure 1 you can see both reactors in comparison.
Figure 1: The large flasks are from our glass workshop department the smaller flasks were bought from the company mentioned above. Single parts of our self-designed H-cell reactors: 1 Custom designed lids that provide connections for: a pO2-electrode, a pH-electrode, an entrance for reference and working electode, air output, heating coils and acid/ base input for pH control, 2 Heating coils, 3 Clamps for the flange connection 4 Sealing rings.
In addition to the H-cell design we thought of an alternative reactor design that meets with the requirements of direct electron transfer. To enable direct electron transfer it is necessary that there is a large electrode surface provided to the microorganisms. Furthermore substrate limitation should be avoided. To meet with these requirements it is favourable to have an reactor that can be continiously driven. Our proposed solution is a flow cell reactor (FCR) which could be driven continiously.
Testing the set up
Our first experiments were carried out with a constant power supply and we measured the voltage input and the current. The set up is shown in figure 2.
It turned out that we could not use the pH-electrode and the pO2-electrode during our cultivations, because they affected the measurement. Especially the pO2-electrode was not suitable in this set up, due to the fact that it is completely made of steel. It turned out that the electrode achieved a grounding of the system which set the lid under electric power. This resulted in a couple of unwanted oxidation processes at the weldseam of the lid. The consequence was to remove both electrodes from the system.
After the customization of the system we carried out a few test runs with differetn electrode materials. At this stage of the project we optimized the attachment of the electrodes and the isolation of the wire which was layed within a silicon tube through the lid.
THe first experiments showed that neutral red is reducable within out set up. The problems that occure if you work with a constant power supply are that the cell potential can not be kept at the same level during the experiments. The dynamic of the electrochemical reactions introduce unwelcome variabilities that cause fluctuations in the potential. Especially the presence of proliferating microorganisms can enhance this effect.
Different electrode materials
We tested different electrode materials for their potential to work in our reactor. We decided to investigate fabric carbon, fabric fleece and platinum electrodes. The different materials are shown in figure 3.
Carbon fabric is made up of individual fibres and has therefore a good stability. Another advantage is that the fibres can overcome quite a long distance due to the fact that they are made of one piece. This assures a good electrical conductivity.
The carbon fleece instead is thicker and provides a larger surface for the microorganisms to attach to the electrode material. This advantage goes at expense of stability and conductivity. The fleece is made of lots of single fibres which leads to a bad connection between them and therefore causes an unfavourable conductivity.
It turned out that platinum was the most suitable material for our experiments.
Cultivation - mediator toxicity test
To evaluate the effect of the mediator cultivations in M9-media with glucose supplemented with 100 µM neutral red or 100 µM bromphenol blue was performed. For the comparison of the growth between the wildtype with and without the mediators samples for OD600 measurement were taken regularly. Figure 4 and 5 show that the mediator has no grave effect on the growth due to the fact that the final OD600 of all cultivations reach similar values. Figure 6 reveals that there is even no big difference between neutral red and bromphenol blue in view of the measured OD600.
Cultivation - constant voltage
The first experiments in the H-cell reactor were performed under constant direct current. These experiments were carried out to test the set up with microorganisms. We investigated if E. coli was able to grow within the needed voltage range and if the different mediators influence the cells if a small electric current is applied.
Figure 7: Comparisson of the growth compatibility of the E. coli KRX WT strain when a voltage is applied or not. Both cultivations were performed in the H-cell reactor in M9 minimal media- xylose (50 mM). One of the cultivatons was performed with an applied voltage of -330 mV the other one was done without voltage. The optical density and the Xylose concentration were measured with technical duplicates.
These results lead to the conclusion that E. coli is not affected in growth by an applied voltage.
A difference can be observed in the growth between the E. coli wildtype and the constructed E. coli ΔdcuB::oprF when both strains are cultivated with a constant voltage of -330 mV. Both strains were cultivated in the H-cell reactor in M9 minimal media- xylose (50 mM) that was supplemented with neutral red to a final concentration of 100 µM.
Figure 8: Comparison of the growth of the E. coli KRX WT strain and the constructed E. coli ΔdcuB::oprF. Both strains were cultivated with a constant voltage of -330 mV in the H-cell reactor in M9 minimal media- xylose (50 mM) with 100 µM neutral red added. The optical density and the Xylose concentration were measured with technical duplicates.
Maybe this effect occures due to the added mediator. To give a valid statement on this effect more effort has to be made on this subject. In our case the result indicates that neutral red might have a positive effect on the growth of our constructed E. coli strain.
Cyclic voltammetry - mediator characterization
The next improvement step in our experiments was to carry out cyclic voltammetry measurments. During our reasearch we found out that the workgroup from Dr. Dirk Holtmann of the Dechema research institute in Frankfurt investigates electroactive microorganisms. We visited them in their laboratory and gained lots of helpful recommendations. THey told us to use a potentiostat for further cultivations and helped us to organize one for our project.
A potentiostat balances the current flow and secures to work at a constant potential. It also functions as a measuring system and therefore provides a way to give a statement if the cells consume electric current.
For our experiments we used a Ag/AgCl reference electrode for measuring the working electrode potential. The counter electrode, which completes the cell circuit, was made from platinum wire. Platinum has the advantage that it is an inert conducter. The set up for the characterization of different mediators is shown is figure 6.
The aim was to detect the potentials were the mediator gets reduced and where it gets oxidized again. We were interested in the potential where the mediator gets reduced, because that potential complies with the conditions where we need to carry out our cultivations.
Furthermore cyclovoltammogramms allow it to give a statement if the redox-reaction is reversible or not. For our measurements we varried the electrode material, the scan-rate, the step-size, the scan-limit and the positioning of the electrodes. In addition we investigated the influence of oxygen in the experimental set-up.
For oxygen free measurements we fumigated the cathode space with nitrogen for approximately 8 hours.
Parameter | Value |
---|---|
Mediator | Bromphenole blue |
Scan rate [mV-s] | 10 |
Step size [mV] | 1 |
Scan limit E1 [V] | 0.4 |
Scan limit E2 [V] | -0.85 |
Electrode material | Platinum |
Aeriation | Oxygen is present |
The cyclic voltammogramm shows that a reversible reaction takes place. In literature you find a value of -739 mV for the reduction of bromphenol blue.(Strehlitz et al., 1994)
Our measurement does not show an reduction peak at this value. That is why have decided not use bpb as mediator. Another reason why we did not use bpb was that its redox potential is very close to the potential where water gets electrolysed. Furthermore we have not tested if E. coli can still grow at such a negative potential.
Parameter | Value |
---|---|
Mediator | Neutral red |
Scan rate [mV-s] | 20 |
Step size [mV] | 1 |
Scan limit E1 [V] | 0.51 |
Scan limit E2 [V] | -0.8 |
Electrode material | Platinum |
Aeriation | Oxygen is present |
In figure 8 are two oxidations peaks present due to presence of oxygen. The small scan rate and step size result in a very flat curve. THe reduction peak is at a similar potential as it is in figure 10 which leads to the assumption that buffer components are reduced and oxidized. The potential where these reactions take place might overlax the reduction peak of neutral read. The redox potential of neutral red accounts to -325 mV vs. standard hydrogen electrode.(Futz, M. L. & Durst, R. A., 1982)
Parameter | Value |
---|---|
Mediator | Neutral red |
Scan rate [mV-s] | 10 |
Step size [mV] | 1 |
Scan limit E1 [V] | 0.1 |
Scan limit E2 [V] | -0.6 |
Electrode material | Platinum |
Aeriation | Oxygen free by aeriation with nitrogen |
Multiple measure cycles were performed to proof if the mediator properties change over the time. The measurement shows that the redox-reaction of neutral red seems to be stable.
Parameter | Value |
---|---|
Mediator | Neutral red in M9 minimal media- xylose (50 mM) with neutral red |
Scan rate [mV-s] | 10 |
Step size [mV] | 1 |
Scan limit E1 [V] | 0.7 |
Scan limit E2 [V] | -0.6 |
Electrode material | Platinum |
Aeriation | Oxygen present |
The measurement shown in figure 13 was performed in M9 minimal-media. We wanted to be sure that neutral red shows a similar redox-reactions in the media we used for the following cultivations.
Chronoamperometry - current consumption
All cultivations were carried out in the H-cell reactor at 37 °C and an air flow of 0.75 standard litres per minute. The used media was M9 minimal media with 50 mM Xylose as carbon source.
The technology of chronoamperometric measurements allows it to tell how much current was needed to keep a set potential constant. The amount of current that is necessary to hold the potential allows conclusion on the energ consumption of the cells.
An additionally performed analytical method was the GloAssay to detect the NAD+ and NADH levels in the cells. This should give hints to the state of the cell metabolism.
Figure 14: Cultivation of the E. coli KRX ΔdcuB::oprF strain in M9 minimal media- xylose (50 mM) with 100 µM neutral red added. During the cultivation there was set a potential of -400 mV on the H-cell achieved by the chronoamperometric method. The figure shows the optical density, Xylose concentration, and the NAD/NADH level during the cultivation, plotted against time.
Figure 15: Cultivation of the E. coli KRX WT in M9 minimal media with 100 µM neutral red added. During the cultivation there was set a potential of -400 mV on the H-cell achieved by the chronoamperometric method. The figure shows the optical density, Xylose concentration, and the NAD/NADH level during the cultivation, plotted against time.
To compare these results we cultivated the E- coli KRX wild type as a reference. The results are shown in figure 16.
Figure 16: Cultivation of the E. coli KRX WT in M9 minimal media with 100 µM neutral red added. During the cultivation there was set a potential of -400 mV on the H-cell achieved by the chronoamperometric method. The figure shows the optical density, Xylose concentration, and the NAD/NADH level during the cultivation, plotted against time.
As an outlook approach more biological replicates should be carried out.
Flow Cell
The figures 18 to 20 show the set up and parts of our FCR. Unfortunately we were not able to use it, because we could't finish our cytochrome construct.
References
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Park, D. H.,Laivenieks, M., Guettler, M. V., Jain, M. K. & Zeikus, J.G. (1999) Microbial utilization of electrically reduced neutral red as the sole electron donor for growth and metabolic production. In: Appl. Environ. Microbiol., 65 (7), pp. 2912 - 2917.
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Strehlitz, B., Gründig, B., Vorlop, K.-D., Bartholmes, P., Kotte, H., Stottmeister, U. (1994) Artificial electron donors for nitrate and nitrite reductases usable as mediators in amperometric biosensors. In: Fresenius' Journal of Analytical Chemistry, 349, pp. 676-678.
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Fultz, M. L., Durst, R. A. (1982): Mediator compounds for the electrochemical study of biological redox systems: a compilation Analytica Chimica Acta. ,140, pp. 1-18