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 CCHHEEMMIICCAALL  EENNGGIINNEEEERRIINNGG  TTRRAANNSSAACCTTIIOONNSS  
 

VOL. 41, 2014 

A publication of 

The Italian Association 
of Chemical Engineering 

www.aidic.it/cet 
Guest Editors: Simonetta Palmas, Michele Mascia, Annalisa Vacca
Copyright © 2014, AIDIC Servizi S.r.l., 
ISBN 978-88-95608-32-7; ISSN 2283-9216                                                                                     
 

Electrochemical Investigation of Aerobic Biocathodes at 
Different Poised Potentials: Evidence for Mediated 

Extracellular Electron Transfer 
Edward Milnera, Keith Scotta, Ian Headb, Tom Curtisb, Eileen Yu*a 
aSchool of Chemical Engineering and Advanced Materials, Newcastle University, Newcastle upon Tyne, UK, NE1 7RU 
bSchool of Civil Engineering and Geosciences, NewcastleUniversity, Newcastle upon Tyne, UK, NE1 7RU 
eileen.yu@ncl.ac.uk 

Microbial Fuel Cells (MFCs) are a promising new technology for the conversion of organic wastes to 
electrical energy. They work by oxidising organics at the anode using bacteria, and combining this with the 
Oxygen Reduction Reaction (ORR) at the cathode. Pt and other chemical catalysts have been used at the 
cathode in MFCs. However, their high cost and issues with long term stability could limit their application in 
MFCs. To have a more sustainable MFC system, one idea is to use aerobic bacteria to catalyse the ORR 
at the cathode, which would make the MFC technology cheaper and more robust. Carbon electrodes 
modified with these bacteria lower the overpotential required for ORR, but little is understood about the 
organisms that constitute these biofilms and their mechanisms of electron transfer. In the current work, 
mixed communities of biofilms catalysing the ORR were grown in electrochemical half-cells poised at 
potentials of +200mV and -100mV vs Ag/AgCl and the electrochemical behaviour of these biofilms was 
studied using Cyclic Voltammetry (CV). These investigations suggest a shift in the mechanism of 
Extracellular Electron Transfer (EET) as the potential changes. 
 

1. Introduction 
Microbial Fuel Cells (MFCs) are devices that use bacteria for the conversion of organic waste to electrical 
energy. In an MFC, bacteria donate electrons to an insoluble anode, which travel through an external 
circuit to a cathode electrode where they combine with oxygen and protons to form water. The circuit is 
completed with the passage of protons form the anode to the cathode, and electrical work is possible by 
electrons passing through the external circuit. MFCs are being developed for energy recovery from organic 
wastes, and could potentially be used for domestic wastewater treatment. Around 1.5% of the total energy 
used in the US is used for wastewater treatment (Logan, 2009). Given that as much as 9.3 times the 
energy that exists in the wastewater is used to treat it, technologies for energy recovery, such as MFCs, 
are vital for future water sustainability (Logan, 2009) 
 
The Oxygen Reduction Reaction (ORR) has slow kinetics on the surface of graphite/carbon cathode 
electrodes, and so expensive, unsustainable precious metal catalysts such as Pt are required to catalyse 
the reaction (Yu et al., 2007). Aerobic biocathodes are a cheap, self-regenerating catalyst, so much 
research in recent years has focused on their development for MFCs (He and Angenent, 2006). An 
aerobic biocathode is a biofilm of a mixed community containing autotrophic, electrotrophic bacteria which 
use the electrode as part of their energy metabolism. They directly accept electrons from poised potential 
electrodes and use these to reduce O2 as part of an electron transport chain in order to generate ATP (Ter 
Heijne et al., 2010). However, very little is known about the dominant electrotrophic organisms in these 
biofilms and their mechanisms of electron transfer, although extracellular electron transfer is thought to 
occur by two different mechanisms; Direct Electron Transfer (DET) via membrane-bound structures such 
as cytochromes, or by Mediated Electron Transfer (MET) via electron mediators (Rosenbaum et al., 2011). 

                                                                                                                                                      
 
 
 
 

          DOI: 10.3303/CET1441060 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 

Please cite this article as: Milner E., Scott K., Head I., Curtis T., Yu E., 2014, Aerobic biocathodes for microbial fuel cells, Chemical 
Engineering Transactions, 41, 355-360  DOI: 10.3303/CET1441060

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The mechanisms established for anode biofilms vary between species. For example, Fe-reducing bacteria 
such as Shewanella oneidensis MR-1 are known to produce electron shuttles (Marsili et al., 2008), 
whereas Fe-reducing Geobacteraceae do not appear to produce electron shuttles and are thought to 
require direct contact with the electrode surface (Bond and Lovley, 2003). Recently, it has been suggested 
that Shewanella oneidensis MR-1 switches from DET to MET depending on the potential of the electrode 
(Roy et al., 2014).  
 
Trying to determine which mechanisms of electron transfer aerobic electrotrophic bacteria use at the 
surface of electrodes is key to understanding aerobic biocathodes in general and to the development of 
the MFC technology as a whole. In the current study therefore, aerobic biocathodes were grown on 
potentiostatically-poised carbon electrodes at two different potentials; -100mV and +200mV vs Ag/AgCl. 
This was done in order to understand the electrochemical behaviour of the biocathodes and establish 
information regarding the mechanism of electron transfer at the electrode surface. The resulting aerobic 
biocathode biofilms were investigated by Cyclic Voltammetry (CV) which is a powerful method for gaining 
mechanistic information about electrochemical processes occurring at electrodes. 

2. Methodology 
2.1 Cell setup, Inoculation and Operation 
3-electrode half-cells for enrichment and study of aerobic biocathode biofilms were assembled. They each 
contained a Working Electrode (WE), Counter Electrode (CE) and Reference Electrode (RE). The WE was 
constructed by attaching a piece of acetone washed carbon felt (2.5 x 5 x 0.5 cm) to a graphite plate 
current collector using a PTFE holder with PTFE screw bolts. Only one side of the CF was exposed to 
electrolyte, and the other pressed up against the graphite plate current collector. The CE was piece of 
coarse platinized mesh of 20 cm2 geometric area and used a Ti wire current collector. The RE assembly 
was made by slotting a glass Ag/AgCl RE purchased from Pine Research Instrumentation through a 
rubber bung and sealing this inside a conical polypropylene tube filled with a 3M NaCl agar gel. Unless 
otherwise stated, all potentials stated in this paper were recorded against the Ag/AgCl reference electrode. 
The half-cell chamber body was made from polypropylene with various ports for the WE, CE and RE. The 
chamber also had a sampling port and gas inlet and outlet ports. The reactor volume was 1L and the WE 
and CE electrode spacing was approximately 2cm.  
 
At the beginning of the experiment, the half-cell chamber was filled with 1L of a trace nutrient medium 
adapted from Ter Heijne et al. (Ter Heijne et al., 2010) for the growth of aerobic biocathode biofilms and 
containing the following; 50mM pH 5.8 phosphate buffer, 10ml/L of a macro nutrients solution, 1ml/L of a 
micro nutrients solution and 1ml/L of a vitamin solution. This trace medium was inoculated using 10% by V 
of activated sludge inoculum obtained from Tudhoe wastewater treatment plant which is located in the 
North East of the UK. The macronutrients solution contained 28g/L NH4Cl, 10g/L MgSO4.7H2O, and 
0.57g/L CaCl2.2H2O. The micro nutrients solution contained 2g/L FeCl2.4H2O, 1g/L CoCl2.6H2O, 0.5g/L 
MnCl2.4H2O, 0.05g/L ZnCl2, 0.05g/L H3BO3, 0.04g/L CuCl2.2H2O, 0.07g/L (NH4)6Mo7O24·4H2O, 1g/L 
NiCl2.6H2O, 0.16 g/L Na2SeO3·5H2O and 2ml/L 37% HCl. The vitamin solution contained 1g/L 
pyridoxine.HCl, 0.5g/L nicotinic acid, 0.25g/L riboflavin, 0.25g/L thiamine.HCl, 0.2g/L biotin, 0.2g/L folic 
acid and 0.01g/L vitamin B12. The cell was then hooked up to a Sycopel potentiostat and the WE 
polarised at -100mV vs. Ag/AgCl. The current was then measured every day. Through the gas inlet, a gas 
sparger was inserted to provide continuous aeration from an aquarium pump. The medium was changed 
for fresh biocathode growth medium every 2-3 weeks. When the medium was changed in the cell, the RE 
drift, pH and OCP were also measured.  
 

2.2 Cyclic Voltammetry (CV) 
The half-cell WEs were characterised by Cyclic Voltammetry (CV) at the beginning of the experiment in the 
non-inoculated medium. CV was performed on an AUTOLAB PGSTAT302 potentiostat by scanning the 
electrode from +500mV to -200mV at a rate of 5mV/s in quiescent non-stirred solution and 4 scans were 
taken for each CV experiment, with the 4th scan taken as the stabilized CV response. At 83 days, the 
carbon felt electrodes were again assessed by CV in exactly the same way. After the biocathode biofilm 
was enriched in the electrochemical half-cell, a third identical half-cell was setup and inoculated using 
effluent from the first. When this cell developed an aerobic biocathode, it was assessed by CV in the same 
way as before. This cell was then sparging with N2 for 1hr whilst the WE was polarised at -100mV in order 
to remove all dissolved O2 from the electrolyte. After removing dissolved O2, an N2 blanket was maintained 
on the surface of the electrolyte, and a series of CV scans were carried out at increasing scan rates from 

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1mV/s to 100mV/s over a range of +500mV to -200mV. At each scan rate, two scans were taken and the 
second scan was taken as the stabilised response. For the CV at different scan rates in the absence of O2, 
a reduction peak and oxidation peak were observed. For the reduction peak, the scan rate and square root 
of the scan rate were plotted separately against the peak height. The peak heights were corrected for 
capacitance by subtracting a linear baseline extrapolated from a capacitive region of the curve. 
 

3. Results and Discussion 
The half-cell started exhibiting increased reduction current above the background ORR current from 
carbon after 50 days of operation, as observed in the CA graph (Figure 1). This increase in performance 
was attributed to the formation of a biocathode biofilm containing electrotrophic aerobic bacteria which are 
able to use the electrode to gain metabolic energy and act as catalysts for the ORR. The electrochemical 
performance of the cell was assessed by CV at the beginning and at 83 days of operation (Figure 1). In 
comparison, the electrode performance increased considerably above the non-inoculated cell containing 
just the carbon electrode in the process electrolyte. The Open Circuit Potential (OCP) of the electrode at 
83 days after inoculation was +460mV and the onset potential for the ORR occurred at values which were 
slightly less than this. In comparison, the non-inoculated cell at the beginning of the experiment had an 
OCP of +100mV and an onset potential for ORR of -100mV. Another key feature of the CV was the 
presence of a double wave in the reduction current as the potential was swept from +500mV to -200mV, 
which was accompanied by a peak on the reverse scan. 
 
 

Figure 1: CA graph showing growth of an electrotrophic aerobic biocathode biofilm on a carbon felt 
electrode polarised at -0.1V vs Ag/AgCl (Top Left). CV of the blank carbon felt electrode at t = 0 days (Top 
Right). CV at t = 0 days and t = 83 days for this carbon felt electrode, showing biocathode formation 
(Bottom).  

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In order to confirm this result, a second cell using effluent from the first was enriched for a biocathode 
biofilm. This cell took 5 days to enrich and was assessed by CV during operation at 41, 50, 103 and 104 
days after inoculation. This cell exhibited the same CA profile, CV and OCP as the biofilms initially 
inoculated from activated sludge, and the CV for this biofilm at 103 days after inoculation is presented in 
Figure 2. O2 was removed from this cell by sparging with N2 and polarising the electrode at -100mV for 1 
hour, and the CV was recorded again. When this was done, the first wave corresponding to ORR by the 
biocathode was removed and the second reduction peak and the oxidation peak remained. This reduction 
and oxidation peak had the same area in the CV, thus showing that they were part of the same redox 
couple. Further to this, the mid-point potential for this redox couple was estimated at +100mV by taking the 
average of the two peak positions.  
 
 
 

 

Figure 2: CV of a biocathode biofilm taken at 103 days after inoculation in aerated solution (solid line) and 
in non-aerated solution (dashed line) 

In the absence of O2, the WE was cycled at increasing scan rates from 1mV/s to 100mV/s, and the peak 
height plotted against the scan rate and the square root of the scan rate (Figure 3). Linearity in the graph 
when the peak height is plotted against the square root of the scan rate indicates semi-infinite diffusion, 
whereas linearity when the peak height is plotted against the scan rate indicates that the redox species are 
absorbed on the surface of the electrode (Léger and Bertrand, 2008). In the case of this cell, the same 
result was demonstrated on 4 separate occasions; the peak height was linear with the square root of the 
scan rate, indicating semi-infinite diffusion. This suggests that in the case of the electrode polarised at -
100mV, there is an electroactive redox species present in the biofilm which is both diffusible and 
reversible, suggesting the presence of an electron mediator which can enable the biofilm to accept 
electrons indirectly from the electrode. This redox active diffusible species could not be detected 
separately in the CV of abiotic carbon electrodes in the electrolyte from the half-cell containing the 
biocathode electrode, suggesting that the diffusible redox active species was confined within the biofilm 
matrix.  
 
 
 

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Figure 3: Peak height for the reduction peak observed in the CV for the aerobic biocathode grown at -
100mV in the absence of air vs scan rate (left) and vs the square root of the scan rate (right) at scan rates 
increasing from 1 to 100mV/s. The CV were recorded and analysed at t = 41, 50, 103 and 104 days after 
inoculation 

In order to provide further evidence for this hypothesis, an identical cell was inoculated from the original 
half-cell, but this cell was polarised at +200mV, a potential where the biofilm would not be able to use a 
mediator with a mid-point potential of +100mV. This third cell developed an aerobic biocathode in exactly 
the same way as the previous two cells, but analysis of the electrode by CV at 26 days after inoculation in 
air and in the absence of air after N2 sparging shows that the resulting aerobic biocathode exhibits none of 
the redox features previously observed (Figure 4). In common with the electrodes polarised at -100mV, the 
electrode polarised at +200mV also exhibited a large positive OCP of +460mV and an onset potential for 
ORR occurring at values slightly less than this. 
 
 
 

 

Figure 4: CV in air (solid line) and in the absence of air (dashed line) for a biocathode grown at a potential 
of +200mV.  

4. Conclusions 
In terms of the energy available for the electrotrophic bacteria within the biocathode biofilm, this is greater 
at the lower potential of -100mV, as compared to an electrode polarised at +200mV, as the potential of O2 
reduction as the terminal electron acceptor for the bacteria at pH 5.8 is 670mV. At -100mV, there is 
evidence for a soluble redox species present in the vicinity of the electrode surface, whereas at +200mV, 
there are no additional redox features observed in the CV. All the biofilms in this study set an OCP of 
+460mV and the onset potential for ORR occurred at values slightly less than this. The presence of a 

359



diffusible species at lower electrode potentials suggests a shift in mechanism to mediated electron transfer 
by the biofilm. The reasons for this could be that there is a competitive advantage for the bacteria in 
switching from DET to MET when the electrode potential is far away from the potential of the redox 
enzyme used by the bacteria. For example, the kinetics of mediated enzyme electrocatalysts are 
influenced by the electron transfer driving force according to; 
 
∆ET = E

0’
enz - E

0’
m (1) 

 
Where E0’enz is the formal redox potential of the enzyme and E

0’
m is the formal redox potential of the 

mediator (Chakraborty and Barton, 2011). As the redox potential of the mediator is shifted further from the 
redox potential of the active site, the rate of enzyme-mediator electron transfer rate increases 
exponentially due to the increased driving force (Kavanagh and Leech, 2013). This might give the aerobic 
biocathode microbes an effective means of utilising the additional energy available from the electrode by 
utilising a mediator with a mid-point potential which is close to the electrode poised potential. More 
effective use of the energy available from the electrode confers a survival advantage in these bacteria over 
other species present in the biofilm. 
 

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