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Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716
Maddalwar and Shanware, 2018
DOI:10.21276/ijlssr.2018.4.6.7
Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2111
Growth Curve Analysis of Rhizobium leguminosarum Using Voltage
Produced by Microbial Fuel Cell
Shrirang R. Maddalwar
1*
, Arti S. Shanware
2
1
Student, Department of Biotechnology, Rajiv Gandhi Biotechnology Centre, Nagpur, India
2
Director, Department of Biotechnology, Rajiv Gandhi Biotechnology Centre, Nagpur, India
*Address for Correspondence: Mr. Shrirang R. Maddalwar, Student, Department of Biotechnology, Rajiv Gandhi
Biotechnology Centre, Nagpur-440020, India
Received: 03 Apr 2018/ Revised: 13 Jul 2018/ Accepted: 16 Oct 2018
ABSTRACT
Microbial fuel cells could be used to the study growth rates of aerobic microbial species on the basis of voltage produced by them
in the microbial fuel cell assembly. A fresh culture of Rhizobium leguminosarum was added in the anode chamber of a microbial
fuel cell assembly and subsequent voltage produced by it was recorded after every fifteen minutes. The 24 ml/hr of air was
pumped in the anode chamber to maintain the dissolved oxygen level and resistance of 12 ohm was applied across the electrodes.
This process was studied in triplicates and voltage data was recorded. The graph plotted of voltage against time suggested the
growth curve of the species in the microbial fuel cell system. It was found that voltage gradually increased with time ranging from
50 mV to 190 mV with a supply of oxygen in the anode, but it declines gradually to zero in absence of aeration with time and
depletion of nutrients.
Key-words Rhizobium leguminosarum, Exo-electrogenesis, Microbial fuel cell, Sporulation, Proton exchange membrane
INTRODUCTION
It is really difficult task to study metabolic activities of a
single bacterial cell, hence in order to avoid this problem
the culture is usually manipulated in such a way that all
the cells of culture should be showing same metabolic
activities. This method is very useful in physiological
studies and also known as synchronous culture method
[1-3]
. A study of these cells would enable one to postulate
the sequence of events occurring in a single cell during
the process of sporulation [4]
. Though this method is very
effective to study the metabolic activities of Rhizobium
leguminosarum but it fails to convey the required
information when the culture is not synchronous[5]
.
A Microbial Fuel Cell (MFC) is a device that converts
chemical energy from bio-convertible organic substrate,
directly into electrical energy through the metabolic
activity of microorganisms.
How to cite this article
Maddalwar SR, Shanware AS. Growth Curve Analysis of Rhizobium
leguminosarum Using Voltage Produced by Microbial Fuel Cell. Int.
J. Life. Sci. Scienti. Res., 2018; 4(6): 2111-2115.
Access this article online
www.ijlssr.com
A simple MFC setup contains two chambers respectively
anode and cathode separated by Proton Exchange
Membrane (PEM). The microorganisms are inoculated in
an anodic chamber, where they oxidize the substrate and
generate protons and electrons. The electrons are
transferred from anode to cathode through the external
circuit and the protons pass through the proton
exchange membrane to cathode, where the proton
meets the oxygen and electrons to form water [6]
.
Mechanism of electron transformation from bacterial
cell to the anode is known by three ways, firstly, using
exogenous mediators (those present outside the cell)
such as thionine, methylene blue or neutral red and
potassium ferricyanide. Secondly, using mediators
produced by the bacteria and finally by direct transfer of
electrons from the respiratory chain enzymes i.e.
cytochromes to the outer cell membrane, which in turn
is reduced and then leaving it in a reduced state to
shuttle the electrons to the electrode [7]
. Geobacter
sulfurreducens, Geobacter metallireducens, and
Rhodoferax ferrireducens have been shown to produce
the voltage in a mediator less microbial fuel cell [8]
.
Hence, in order to study metabolic activities of
Rhizobium leguminosarum in liquid broth, the microbial
Research Article
Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716
Maddalwar and Shanware, 2018
DOI:10.21276/ijlssr.2018.4.6.7
Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2112
fuel cell could be used as an effective tool. This study
focuses on voltage generated by the microbial fuel cell
using fresh broth of Rhizobium leguminosarum with
respect to aeration and in absence of aeration. It could
be an effective method to determine the metabolic rate
of cells in different physiological and nutritional
conditions.
MATERIALS AND METHODS
Pre-isolated and pre-characterized culture tube of
Rhizobium leguminosarum from the soil samples Rajiv
Gandhi Biotechnology Centre, Nagpur, India premises
was considered for inoculation of fresh growth medium
in laboratory of Department of Biotechnology at 16
December 2017.
Preparation of fresh culture broth- The fresh nutrient
medium was prepared using Yeast Mannitol medium
(YEMA medium) which includes K2HPO4 0.05%, MgSO4
0.02%, NaCl 0.01%, Mannitol 1%, CaCO3 0.3%, Yeast 0.1%
and Distilled water. The contents of the medium are
thoroughly mixed and allowed for autoclaving at 121O
C
and 15 lb pressure. After the process of autoclaving the
medium, the medium is allowed to settle down to room
temperature. This process can be done more rapidly by
placing the container of nutrient medium in cool stream
of water. Once the content is cooled then pH of the
medium was measured using digital pH meter. The
optimum pH of this medium for Rhizobium species
should be 7 and hence it is necessary to confirm it. If the
pH is not neutral, then it is made neutral by adding
strong acid like HCl or strong base like NaOH. After
gaining optimum pH, the broth was inoculated with 10%
inoculums of a Rhizobium leguminosarum and the
content was allowed to grow in well-aerated desktop
fermentor or cotton-plugged glass flask. Culture requires
oxygen to multiply and grow efficiently; hence aerobic
fermentor is always preferable. The medium was allowed
to grow for next 48 hours [9]
.
Microbial fuel cell construction- The MFC was
constructed using two screw-capped plastic bottles with
the total working volume of 1 liter and it served as anode
(anaerobic) and cathode (aerobic) chambers. Both anode
and cathode chambers were connected with 1 cm in
diameter and 5 cm long tube which was filled up with
salt bridge made of 1M Potassium chloride (KCl) solution
and 3% agar powder. Agar salt bridge acts as a barrier
between the anode and cathode chambers. The reason
for using agars as salt bridge is to provide an internal
electrical connection between the chambers, while
minimizing the transfer of ions from the electrical
environment [10]
. Stainless steel mesh of 500 gm and
having diameter of 2 mm was used as anode and
cathode. Before the MFC operation, the electrodes were
soaked in 0.1 M HCl solution for a day to remove
possible contamination and after the MFC operation the
electrodes were washed with 0.1 M NaOH solution to
neutralize the surface contaminants [11]
. The electrodes
were externally connected with 12 ohm resistance using
copper wire. This setup was prepared in triplicates in
order to minimize the errors in voltage recorded by the
volt meter. Aeration of 600 ml per hour is supplied to the
cathode chamber using 1 liter injection syringe. Both the
bottles are screw capped properly in order to make both
the chambers air tight.
Microbial fuel cell operation- All the three microbial fuel
cell setups are surface sterilized by wiping with 70%
alcohol and UV light exposure for 20 minutes. All the
three anode chambers of microbial fuel cell assemblies
were filled with 400 ml freshly prepared broth culture of
Rhizobium leguminosarum in each chamber. After
inoculation, the assemblies are screw capped properly to
maintain anaerobic conditions inside the chamber. In
cathode chamber, 800 ml of 1 M KCl solution was filled
in all the three assemblies. All the three assemblies are
screw capped and aeration of 600 ml per hour is
provided to the assemblies using 1 liter injection syringe.
Whatman filter is attached to the syringe before aeration
in order to provide sterile air flow [9]
.
RESULTS
A resistance of 12 ohm is applied across cathodes and
anodes of each assembly and voltage is recorded in the
voltmeter after every fifteen minutes. After one hour
and 45 minutes, the aeration is stopped and voltage is
recorded after every 15 minutes for five more times
successively. Detailed data of recorded voltage in mV is
summarized in Table 1 and Fig. 1.
Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716
Maddalwar and Shanware, 2018
DOI:10.21276/ijlssr.2018.4.6.7
Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2113
Table 1: Voltage recorded by three microbial fuel cell assemblies after every 15 minutes
Time (Minutes)
Voltage recorded by Set
A (mV)
Voltage recorded by Set B
(mV)
Voltage recorded by Set C
(mV)
0 90 50 70
15 130 70 100
30 130 90 120
45 160 108 127
60 185 130 135
75 184 145 150
90 184 180 182
105 184 180 182
AERATION STOPPED
120 190 190 180
135 180 190 170
150 150 180 120
165 140 144 108
180 130 25 80
195 10 00 00
Fig. 1: Voltage produced by the culture of Rhizobium species with respect to time
Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716
Maddalwar and Shanware, 2018
DOI:10.21276/ijlssr.2018.4.6.7
Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2114
DISCUSSION
There has been an increase in recent years in the
number of reports of microorganisms that can generate
electrical current in microbial fuel cells. Although many
new strains have been identified, few strains individually
produce power densities as high as strains from mixed
communities. Enriched anodic bio-films have generated
power densities as high as 6.9 W per m2
(projected
anode area), and therefore are approaching theoretical
limits [12]
.
Power density, electrode potential, coulombic efficiency,
and energy recovery in single-chamber microbial fuel
cells (MFCs) were examined as a function of solution
ionic strength, electrode spacing and composition, and
temperature. By the increasing the solution ionic
strength from 100 to 400 mM by adding NaCl increased
power output from 720 to 1330 mW/m2
. Power
generation was also increased from 720 to 1210 mW/m2
by decreasing the distance between the anode and
cathode from 4 to 2 cm. The power increases due to
ionic strength and electrode spacing resulted from a
decrease in the internal resistance. Power output was
also increased by 68% by replacing the cathode
(purchased from a manufacturer) with carbon cloth
cathode containing the Pt loading[13]
.
It is a surprise to many researchers that the most
significant block to achieving high power densities in
MFCs is the system architecture, not the composition of
the bacterial community [14]
.
But power output by MFCs has been consistently
increasing over time. Improvements in system
architecture and operation have increased power
densities from 1500 mW/m2
using oxygen as the final
electron acceptor at the cathode [15,16].
From Fig. 1 and Table 1 were observed that the voltage
produced by a freshly prepared broth of Rhizobium
leguminosarum increases with time from its actual value
to 180-190 mV with aeration of 600 ml per hour of
sterile air in cathode chamber in 105 minutes. But when
the aeration is stopped completely, the voltage
produced by the culture in microbial fuel cell setup also
decreases gradually and it becomes zero after 180
minutes of starting the experiment. This change in
voltage with respect to time and with respect to aeration
observed in very similar pattern in all the three sets
namely A, B, and C or microbial fuel cell assembly.
Hence, the graph of voltage against time gradually
increases with aeration and it gradually decreases from
the peak when the aeration is stopped in the cathode
chamber of microbial fuel cell assemblies. The graph
declines to zero after 180 minutes.
The increase in the voltage generated by microbial fuel
cells with aeration suggests that metabolic rate of the
growing culture in the anode chamber increased with
aeration, but after stoppage of aeration, the metabolic
rate of the bacterial culture decreased gradually due to
insufficiency of oxygen in the cathode chamber and as a
result voltage produced by it also decreased and it
become zero after 195 minutes of experiment when
oxygen was completely exhausted in the cathode
chamber. Zero voltage recorded by microbial fuel cell
assemblies suggests that the fuel cell stops working and
cells in the culture might have died.
CONCLUSIONS
From this study it could be concluded that pre-isolated
strain of R. leguminosarum is highly aerobic in nature
and require enough oxygen to metabolize and
reproduce. The cell behavior or nutrient uptake studies
of R. leguminosarum could be done using the voltage
generated by it in microbial fuel cell assemblies. The
maximum voltage generated by a freshly prepared broth
of R. leguminosarum is in between 180 mV - 190 mV in
microbial fuel cell assembly.
In future, more work is required to be done on the
assembly for increasing this range of voltage. In addition
to this comparative study of different electrode material
can also be done in order to get an efficient and steady
voltage for the sample organism.
ACKNOWLEDGMENTS
This investigation was fulfilled with the continuous
support of all the teaching and non-teaching staff of Rajiv
Gandhi Biotechnology Centre, Nagpur. I am especially
thankful to Dr. Arti S. Shanware for her continuous
guidance and support while undergoing this research
work.
CONTRIBUTION OF AUTHORS
All authors equally contributed to this article.
REFERENCES
[1] Halvorson HO. Physiology of sporulation, In I. C.
Gunsalus and R. Y. Stanier [ed.], the bacteria.
Academic Press, Inc., New York, 1962; 4: 223-274.
Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716
Maddalwar and Shanware, 2018
DOI:10.21276/ijlssr.2018.4.6.7
Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2115
[2] Halvorson HO. Sequential expression of biochemical
events during intracellular differentiation. Symp. Soc.
Gen. Microbiol., 1965; 15: 343-368.
[3] Murrell WG. Spore formation and germination as a
microbial reaction to the environment. Symp. Soc.
Gen. Microbiol., 1961; 11: 100-150.
[4] Microbial fuel cells. USA. John Wiley and Sons, 2008;
pp. 1-125.
[5] Imanaka H, Gillis JR, Slepecky RA. Synchronous
Growth and Sporulation of Bacillus megaterium. J
Bacteriol., 1967; 93(5): 1624-1630.
[6] Sharma Suresh K, Bulchandani BD. Comparative
Study of Various Substrates and Microorganisms in a
Laboratory Designed Microbial Fuel Cell Int. J Res
Chem Environ. 2012; 2(3): 168-174.
[7] Chaudhury SK, Lovely DR. Electricity generation by
direct oxidation of glucose in mediatorless microbial
fuel cells. Nat. Biotechnol., 2003; 21: 1229-1232.
[8] Bond DR, Lovely DR. Electricity production by
Geobacter sulfurreducens attached to electrodes,
Appl Environ Microbiol., 2003; 69: 1548-1555.
[9] Jakaria Al-Mujahidy SK, Hassan M, Rahman M,
Mamun-Or-Rashid ANM. Isolation and
characterization of Rhizobium sp. and determination
of their potency for growth factor production. Int.
Res. J. Biotechnol.,2013; 4(7): 117-123.
[10]Patil VD, Patil DB, Deshmukh MB, Pawar SH.
Comparative study of bioelectricity generation along
with the treatment of different sources of
wastewater. International Journal of Chemical
Sciences and Applications, 2011; 2(2): 162-168.
[11]Liu ZD, Li HR. Effects of Bio and Abio-factors on
Electricity Production in a Mediatorless Microbial
Fuel Cell, Biochem Eng J., 2007; 36(3): 209-214.
[12]Logan BE. Exoelectrogenic bacteria that power
microbial fuel cell. Nature reviews: Microbiology,
2009, pp. 375-381.
[13]Hong Liu, Shaoan Cheng, Logan BE. Power
generation in Fed- Batch Microbial Fuel Cell as a
function of ionic strength, Temperature & Reactor
Configuration. Environ. Sci. Technol. 2005; 39:
5488-5493.
[14] Kim BH, et al. Mediator-less biofuel cell. U.S. Patent
5976719, 1999.
[15]Cheng S, et al. Increased power generation in a
continuous flow MFC with advective flow through
the porous anode and reduced electrode spacing.
Environ. Sci. Technol., 2006; 40: 2426โ€“2432.
[16]Min B, et al. Electricity generation using membrane
and salt bridge microbial fuel cells. Water Res., 2005;
39, 1675โ€“1686.
Open Access Policy:
Authors/Contributors are responsible for originality, contents, correct references, and ethical issues. IJLSSR publishes all articles under Creative
Commons Attribution- Non-Commercial 4.0 International License (CC BY-NC). https://creativecommons.org/licenses/by-nc/4.0/legalcode

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Growth Curve Analysis of Rhizobium leguminosarum Using Voltage Produced by Microbial Fuel Cell

  • 1. Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716 Maddalwar and Shanware, 2018 DOI:10.21276/ijlssr.2018.4.6.7 Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2111 Growth Curve Analysis of Rhizobium leguminosarum Using Voltage Produced by Microbial Fuel Cell Shrirang R. Maddalwar 1* , Arti S. Shanware 2 1 Student, Department of Biotechnology, Rajiv Gandhi Biotechnology Centre, Nagpur, India 2 Director, Department of Biotechnology, Rajiv Gandhi Biotechnology Centre, Nagpur, India *Address for Correspondence: Mr. Shrirang R. Maddalwar, Student, Department of Biotechnology, Rajiv Gandhi Biotechnology Centre, Nagpur-440020, India Received: 03 Apr 2018/ Revised: 13 Jul 2018/ Accepted: 16 Oct 2018 ABSTRACT Microbial fuel cells could be used to the study growth rates of aerobic microbial species on the basis of voltage produced by them in the microbial fuel cell assembly. A fresh culture of Rhizobium leguminosarum was added in the anode chamber of a microbial fuel cell assembly and subsequent voltage produced by it was recorded after every fifteen minutes. The 24 ml/hr of air was pumped in the anode chamber to maintain the dissolved oxygen level and resistance of 12 ohm was applied across the electrodes. This process was studied in triplicates and voltage data was recorded. The graph plotted of voltage against time suggested the growth curve of the species in the microbial fuel cell system. It was found that voltage gradually increased with time ranging from 50 mV to 190 mV with a supply of oxygen in the anode, but it declines gradually to zero in absence of aeration with time and depletion of nutrients. Key-words Rhizobium leguminosarum, Exo-electrogenesis, Microbial fuel cell, Sporulation, Proton exchange membrane INTRODUCTION It is really difficult task to study metabolic activities of a single bacterial cell, hence in order to avoid this problem the culture is usually manipulated in such a way that all the cells of culture should be showing same metabolic activities. This method is very useful in physiological studies and also known as synchronous culture method [1-3] . A study of these cells would enable one to postulate the sequence of events occurring in a single cell during the process of sporulation [4] . Though this method is very effective to study the metabolic activities of Rhizobium leguminosarum but it fails to convey the required information when the culture is not synchronous[5] . A Microbial Fuel Cell (MFC) is a device that converts chemical energy from bio-convertible organic substrate, directly into electrical energy through the metabolic activity of microorganisms. How to cite this article Maddalwar SR, Shanware AS. Growth Curve Analysis of Rhizobium leguminosarum Using Voltage Produced by Microbial Fuel Cell. Int. J. Life. Sci. Scienti. Res., 2018; 4(6): 2111-2115. Access this article online www.ijlssr.com A simple MFC setup contains two chambers respectively anode and cathode separated by Proton Exchange Membrane (PEM). The microorganisms are inoculated in an anodic chamber, where they oxidize the substrate and generate protons and electrons. The electrons are transferred from anode to cathode through the external circuit and the protons pass through the proton exchange membrane to cathode, where the proton meets the oxygen and electrons to form water [6] . Mechanism of electron transformation from bacterial cell to the anode is known by three ways, firstly, using exogenous mediators (those present outside the cell) such as thionine, methylene blue or neutral red and potassium ferricyanide. Secondly, using mediators produced by the bacteria and finally by direct transfer of electrons from the respiratory chain enzymes i.e. cytochromes to the outer cell membrane, which in turn is reduced and then leaving it in a reduced state to shuttle the electrons to the electrode [7] . Geobacter sulfurreducens, Geobacter metallireducens, and Rhodoferax ferrireducens have been shown to produce the voltage in a mediator less microbial fuel cell [8] . Hence, in order to study metabolic activities of Rhizobium leguminosarum in liquid broth, the microbial Research Article
  • 2. Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716 Maddalwar and Shanware, 2018 DOI:10.21276/ijlssr.2018.4.6.7 Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2112 fuel cell could be used as an effective tool. This study focuses on voltage generated by the microbial fuel cell using fresh broth of Rhizobium leguminosarum with respect to aeration and in absence of aeration. It could be an effective method to determine the metabolic rate of cells in different physiological and nutritional conditions. MATERIALS AND METHODS Pre-isolated and pre-characterized culture tube of Rhizobium leguminosarum from the soil samples Rajiv Gandhi Biotechnology Centre, Nagpur, India premises was considered for inoculation of fresh growth medium in laboratory of Department of Biotechnology at 16 December 2017. Preparation of fresh culture broth- The fresh nutrient medium was prepared using Yeast Mannitol medium (YEMA medium) which includes K2HPO4 0.05%, MgSO4 0.02%, NaCl 0.01%, Mannitol 1%, CaCO3 0.3%, Yeast 0.1% and Distilled water. The contents of the medium are thoroughly mixed and allowed for autoclaving at 121O C and 15 lb pressure. After the process of autoclaving the medium, the medium is allowed to settle down to room temperature. This process can be done more rapidly by placing the container of nutrient medium in cool stream of water. Once the content is cooled then pH of the medium was measured using digital pH meter. The optimum pH of this medium for Rhizobium species should be 7 and hence it is necessary to confirm it. If the pH is not neutral, then it is made neutral by adding strong acid like HCl or strong base like NaOH. After gaining optimum pH, the broth was inoculated with 10% inoculums of a Rhizobium leguminosarum and the content was allowed to grow in well-aerated desktop fermentor or cotton-plugged glass flask. Culture requires oxygen to multiply and grow efficiently; hence aerobic fermentor is always preferable. The medium was allowed to grow for next 48 hours [9] . Microbial fuel cell construction- The MFC was constructed using two screw-capped plastic bottles with the total working volume of 1 liter and it served as anode (anaerobic) and cathode (aerobic) chambers. Both anode and cathode chambers were connected with 1 cm in diameter and 5 cm long tube which was filled up with salt bridge made of 1M Potassium chloride (KCl) solution and 3% agar powder. Agar salt bridge acts as a barrier between the anode and cathode chambers. The reason for using agars as salt bridge is to provide an internal electrical connection between the chambers, while minimizing the transfer of ions from the electrical environment [10] . Stainless steel mesh of 500 gm and having diameter of 2 mm was used as anode and cathode. Before the MFC operation, the electrodes were soaked in 0.1 M HCl solution for a day to remove possible contamination and after the MFC operation the electrodes were washed with 0.1 M NaOH solution to neutralize the surface contaminants [11] . The electrodes were externally connected with 12 ohm resistance using copper wire. This setup was prepared in triplicates in order to minimize the errors in voltage recorded by the volt meter. Aeration of 600 ml per hour is supplied to the cathode chamber using 1 liter injection syringe. Both the bottles are screw capped properly in order to make both the chambers air tight. Microbial fuel cell operation- All the three microbial fuel cell setups are surface sterilized by wiping with 70% alcohol and UV light exposure for 20 minutes. All the three anode chambers of microbial fuel cell assemblies were filled with 400 ml freshly prepared broth culture of Rhizobium leguminosarum in each chamber. After inoculation, the assemblies are screw capped properly to maintain anaerobic conditions inside the chamber. In cathode chamber, 800 ml of 1 M KCl solution was filled in all the three assemblies. All the three assemblies are screw capped and aeration of 600 ml per hour is provided to the assemblies using 1 liter injection syringe. Whatman filter is attached to the syringe before aeration in order to provide sterile air flow [9] . RESULTS A resistance of 12 ohm is applied across cathodes and anodes of each assembly and voltage is recorded in the voltmeter after every fifteen minutes. After one hour and 45 minutes, the aeration is stopped and voltage is recorded after every 15 minutes for five more times successively. Detailed data of recorded voltage in mV is summarized in Table 1 and Fig. 1.
  • 3. Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716 Maddalwar and Shanware, 2018 DOI:10.21276/ijlssr.2018.4.6.7 Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2113 Table 1: Voltage recorded by three microbial fuel cell assemblies after every 15 minutes Time (Minutes) Voltage recorded by Set A (mV) Voltage recorded by Set B (mV) Voltage recorded by Set C (mV) 0 90 50 70 15 130 70 100 30 130 90 120 45 160 108 127 60 185 130 135 75 184 145 150 90 184 180 182 105 184 180 182 AERATION STOPPED 120 190 190 180 135 180 190 170 150 150 180 120 165 140 144 108 180 130 25 80 195 10 00 00 Fig. 1: Voltage produced by the culture of Rhizobium species with respect to time
  • 4. Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716 Maddalwar and Shanware, 2018 DOI:10.21276/ijlssr.2018.4.6.7 Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2114 DISCUSSION There has been an increase in recent years in the number of reports of microorganisms that can generate electrical current in microbial fuel cells. Although many new strains have been identified, few strains individually produce power densities as high as strains from mixed communities. Enriched anodic bio-films have generated power densities as high as 6.9 W per m2 (projected anode area), and therefore are approaching theoretical limits [12] . Power density, electrode potential, coulombic efficiency, and energy recovery in single-chamber microbial fuel cells (MFCs) were examined as a function of solution ionic strength, electrode spacing and composition, and temperature. By the increasing the solution ionic strength from 100 to 400 mM by adding NaCl increased power output from 720 to 1330 mW/m2 . Power generation was also increased from 720 to 1210 mW/m2 by decreasing the distance between the anode and cathode from 4 to 2 cm. The power increases due to ionic strength and electrode spacing resulted from a decrease in the internal resistance. Power output was also increased by 68% by replacing the cathode (purchased from a manufacturer) with carbon cloth cathode containing the Pt loading[13] . It is a surprise to many researchers that the most significant block to achieving high power densities in MFCs is the system architecture, not the composition of the bacterial community [14] . But power output by MFCs has been consistently increasing over time. Improvements in system architecture and operation have increased power densities from 1500 mW/m2 using oxygen as the final electron acceptor at the cathode [15,16]. From Fig. 1 and Table 1 were observed that the voltage produced by a freshly prepared broth of Rhizobium leguminosarum increases with time from its actual value to 180-190 mV with aeration of 600 ml per hour of sterile air in cathode chamber in 105 minutes. But when the aeration is stopped completely, the voltage produced by the culture in microbial fuel cell setup also decreases gradually and it becomes zero after 180 minutes of starting the experiment. This change in voltage with respect to time and with respect to aeration observed in very similar pattern in all the three sets namely A, B, and C or microbial fuel cell assembly. Hence, the graph of voltage against time gradually increases with aeration and it gradually decreases from the peak when the aeration is stopped in the cathode chamber of microbial fuel cell assemblies. The graph declines to zero after 180 minutes. The increase in the voltage generated by microbial fuel cells with aeration suggests that metabolic rate of the growing culture in the anode chamber increased with aeration, but after stoppage of aeration, the metabolic rate of the bacterial culture decreased gradually due to insufficiency of oxygen in the cathode chamber and as a result voltage produced by it also decreased and it become zero after 195 minutes of experiment when oxygen was completely exhausted in the cathode chamber. Zero voltage recorded by microbial fuel cell assemblies suggests that the fuel cell stops working and cells in the culture might have died. CONCLUSIONS From this study it could be concluded that pre-isolated strain of R. leguminosarum is highly aerobic in nature and require enough oxygen to metabolize and reproduce. The cell behavior or nutrient uptake studies of R. leguminosarum could be done using the voltage generated by it in microbial fuel cell assemblies. The maximum voltage generated by a freshly prepared broth of R. leguminosarum is in between 180 mV - 190 mV in microbial fuel cell assembly. In future, more work is required to be done on the assembly for increasing this range of voltage. In addition to this comparative study of different electrode material can also be done in order to get an efficient and steady voltage for the sample organism. ACKNOWLEDGMENTS This investigation was fulfilled with the continuous support of all the teaching and non-teaching staff of Rajiv Gandhi Biotechnology Centre, Nagpur. I am especially thankful to Dr. Arti S. Shanware for her continuous guidance and support while undergoing this research work. CONTRIBUTION OF AUTHORS All authors equally contributed to this article. REFERENCES [1] Halvorson HO. Physiology of sporulation, In I. C. Gunsalus and R. Y. Stanier [ed.], the bacteria. Academic Press, Inc., New York, 1962; 4: 223-274.
  • 5. Int. J. Life. Sci. Scienti. Res. eISSN: 2455-1716 Maddalwar and Shanware, 2018 DOI:10.21276/ijlssr.2018.4.6.7 Copyright ยฉ 2015 - 2018| IJLSSR by Society for Scientific Research under a CC BY-NC 4.0 International License Volume 04 | Issue 06 | Page 2115 [2] Halvorson HO. Sequential expression of biochemical events during intracellular differentiation. Symp. Soc. Gen. Microbiol., 1965; 15: 343-368. [3] Murrell WG. Spore formation and germination as a microbial reaction to the environment. Symp. Soc. Gen. Microbiol., 1961; 11: 100-150. [4] Microbial fuel cells. USA. John Wiley and Sons, 2008; pp. 1-125. [5] Imanaka H, Gillis JR, Slepecky RA. Synchronous Growth and Sporulation of Bacillus megaterium. J Bacteriol., 1967; 93(5): 1624-1630. [6] Sharma Suresh K, Bulchandani BD. Comparative Study of Various Substrates and Microorganisms in a Laboratory Designed Microbial Fuel Cell Int. J Res Chem Environ. 2012; 2(3): 168-174. [7] Chaudhury SK, Lovely DR. Electricity generation by direct oxidation of glucose in mediatorless microbial fuel cells. Nat. Biotechnol., 2003; 21: 1229-1232. [8] Bond DR, Lovely DR. Electricity production by Geobacter sulfurreducens attached to electrodes, Appl Environ Microbiol., 2003; 69: 1548-1555. [9] Jakaria Al-Mujahidy SK, Hassan M, Rahman M, Mamun-Or-Rashid ANM. Isolation and characterization of Rhizobium sp. and determination of their potency for growth factor production. Int. Res. J. Biotechnol.,2013; 4(7): 117-123. [10]Patil VD, Patil DB, Deshmukh MB, Pawar SH. Comparative study of bioelectricity generation along with the treatment of different sources of wastewater. International Journal of Chemical Sciences and Applications, 2011; 2(2): 162-168. [11]Liu ZD, Li HR. Effects of Bio and Abio-factors on Electricity Production in a Mediatorless Microbial Fuel Cell, Biochem Eng J., 2007; 36(3): 209-214. [12]Logan BE. Exoelectrogenic bacteria that power microbial fuel cell. Nature reviews: Microbiology, 2009, pp. 375-381. [13]Hong Liu, Shaoan Cheng, Logan BE. Power generation in Fed- Batch Microbial Fuel Cell as a function of ionic strength, Temperature & Reactor Configuration. Environ. Sci. Technol. 2005; 39: 5488-5493. [14] Kim BH, et al. Mediator-less biofuel cell. U.S. Patent 5976719, 1999. [15]Cheng S, et al. Increased power generation in a continuous flow MFC with advective flow through the porous anode and reduced electrode spacing. Environ. Sci. Technol., 2006; 40: 2426โ€“2432. [16]Min B, et al. Electricity generation using membrane and salt bridge microbial fuel cells. Water Res., 2005; 39, 1675โ€“1686. Open Access Policy: Authors/Contributors are responsible for originality, contents, correct references, and ethical issues. IJLSSR publishes all articles under Creative Commons Attribution- Non-Commercial 4.0 International License (CC BY-NC). https://creativecommons.org/licenses/by-nc/4.0/legalcode