Identification of Microbial Communities in Open and Closed Circuit Bioelectrochemical MBRs by High-Throughput 454 Pyrosequencing

Jian Huang; Zhiwei Wang; Chaowei Zhu; Jinxing Ma; Xingran Zhang; Zhichao Wu

doi:10.1371/journal.pone.0093842

Abstract

Two bioelectrochemical membrane bioreactors (MBRs) developed by integrating microbial fuel cell and MBR technology were operated under closed-circuit and open-circuit modes, and high-throughput 454 pyrosequencing was used to investigate the effects of the power generation on the microbial community of bio-anode and bio-cathode. Microbes on the anode under open-circuit operation (A_O) were enriched and highly diverse when compared to those on the anode under closed-circuit operation (A_C). However, among the cathodes the closed-circuit mode (C_C) had richer and more diverse microbial community compared to the cathode under open-circuit mode (C_O). On the anodes A_O and A_C, Proteobacteria and Bacteroidetes were the dominant phyla, while Firmicutes was enriched only on A_C. Deltaproteobacteria affiliated to Proteobacteria were also more abundant on A_C than A_O. Furthermore, the relative abundance of Desulfuromonas, which are well-known electrogenic bacteria, were much higher on A_C (10.2%) when compared to A_O (0.11%), indicating that closed-circuit operation was more conducive for the growth of electrogenic bacteria on the anodes. On the cathodes, Protebacteria was robust on C_C while Bacteroidetes was more abundant on C_O. Rhodobacter and Hydrogenophaga were also enriched on C_C than C_O, suggesting that these genera play a role in electron transfer from the cathode surface to the terminal electron acceptors in the bioelectrochemical MBR under closed-circuit operation.

Citation: Huang J, Wang Z, Zhu C, Ma J, Zhang X, Wu Z (2014) Identification of Microbial Communities in Open and Closed Circuit Bioelectrochemical MBRs by High-Throughput 454 Pyrosequencing. PLoS ONE 9(4): e93842. https://doi.org/10.1371/journal.pone.0093842

Editor: Hauke Smidt, Wageningen University, Netherlands

Received: September 5, 2013; Accepted: March 7, 2014; Published: April 4, 2014

Copyright: © 2014 Huang et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Funding: This work was financially supported by the Science and Technology Commission of Shanghai Municipality project (12230707000) and by the Fundamental Research Funds for the Central Universities. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Microbial fuel cells (MFCs) offer a promising technology for both organic waste treatment and simultaneous power generation, and have attracted attention in the past decade. However, the practical applications of MFCs are limited by disadvantages such as low treatment efficiency and poor effluent quality. Membrane bioreactor (MBR) is another promising wastewater treatment process that has achieved great advances in the past two decades. MBR is considered as an alternate technology for conventional activated sludge (CAS) systems due to its high treatment efficiency and good effluent quality [1]. However, its wide-spread application is hindered by the high energy consumption.

Recently, efforts have been made to integrate MFC and MBR for wastewater treatment. It is presumed that the power generated by MFC from wastewater will partially offset the energy requirement of MBR, which in turn could increase treatment efficiency and enhance effluent quality of MFC. In a recently developed MFC-MBR system the aeration tank of an MBR was used as the cathode chamber [2]. Stainless-steel mesh membrane module has also been used as the cathode in an MFC-MBR system, which achieved a maximum power density of 8.62 W/m³ [3]. In another study, removal of 92.4% chemical oxygen demand (COD) and 4.35 W/m³ power density has also been reported [4]. These studies demonstrate the potential of bioelectrochemical MBR created by MFC-MBR integration for simultaneous wastewater treatment and energy production.

In these integrated systems, microorganisms play critical roles in both power generation and also wastewater treatment. Power is generated when microorganisms on the anode act as catalysts to oxidize organic matters and transfer the generated electrons to the cathode though an external circuit while the microbes on the cathode function as biocatalysts and accept electrons. On the other hand, biological wastewater treatment is generally carried out in the cathode chamber (aerobic MBR basin), which also impacts the microbial community on the cathode. A number of studies have determined the microbial community in typical MFCs [5]–[7]. However, studies on the microbial communities in bioelectrochemical MBRs are limited. Due to the distinct differences between typical MFCs and integrated MFC-MBR systems, the microbes in these newer systems are expected to be unique. Therefore, understanding their composition and functions will allow optimization of these integrated systems.

The goal of this study was to characterize the microbial community in the integrated MFC-MBR systems. To achieve this goal, we developed two identical bioelectrochemical membrane bioreactors (MBRs) by integrating MFC and MBR technology and operated them under closed-circuit and open-circuit modes. We then compared the microbial communities between the two MBRs using high-throughput 454 pyrosequencing to investigate the effects of power generation on microbial community changes on the bio-anode and bio-cathode. The results of this study provide insights into the microbial communities and their functions in MFC-MBR systems, and will facilitate optimization of these integrated systems for efficient wastewater treatment and power generation.

Materials and Methods

Experimental set-up

The schematic diagram of the experimental setup is shown in Fig. 1. The bioelectrochemical MBR was designed to have two cylinder compartments both with the same inner diameter of 10 cm, and designated as the anode and cathode chambers. The two chambers were separated by a cloth pretreated with polyvinylidene fluoride. A 3-cm long Plexiglas tube with 8 mm diameter was installed in the anode chamber to enable continuous upflow of wastewater from anode to the cathode.

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Figure 1. Schematic diagram of the bioelectrochemical MBR system.

(1) Anode chamber; (2) cathode chamber; (3) cloth separating the two chambers; (4) stainless-steel mesh membrane module; (5) influent pipe; (6) effluent pipe; (7) connecting pipe; (8) air diffuser.

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The anode chamber was filled with graphite felts (10-cm diameter) that were cut into pieces of 1 cm×1 cm (width × thickness). Total volume of the anode chamber was 140 mL and the volume of water decreased to 37 mL after the installation of graphite felts. Then, a graphite rod (6 mm diameter) was inserted in the anode graphite felts and connected to the external circuit. The cathode was a flat-sheet membrane (4 cm×8 cm) made of stainless mesh (pore size 48 μm), and was installed in the cathode chamber with an effective volume of 1.25 L. Two graphite rods were fastened on each side of the membrane module using stainless steel wires. Two perforated Plexiglas tubes were mounted below the membrane module to supply oxygen and mix liquids with an aeration intensity of 0.67 L/min.

In the bioelectrochemical MBR under closed-circuit operation (MBR_C), the graphite rods in both anode and cathode were connected with copper wires with 470 or 100 Ω external resistance, while the graphite rods remained open in the MBR under open-circuit operation (MBR_O), which also served as a control reactor. This design enabled us to compare the differences in the microbial communities between the two systems, and analyze the impact of different modes of power generation on variations in the microbial communities.

Inoculation and operation

The anode chambers in both bioelectrochemical MBRs were inoculated with 10 mL sludge obtained from the anaerobic unit of an anaerobic/anoxic/oxic-MBR system, which is documented in a previous publication [8]. The mixed liquor suspended solid (MLSS) and mixed liquor volatile suspended solid (MLVSS) concentrations of the inoculated sludge were 16.2 g/L and 9.0 g/L, respectively. The cathode chambers were seeded with activated sludge from Shanghai Quyang municipal wastewater treatment plant in China, which had an MLSS concentration of 3.9 g/L and an MLVSS concentration of 2.8 g/L.

After inoculation, synthetic wastewater was fed into the anode chamber, and then allowed to flow into the cathode chamber. Composition of the synthetic wastewater was: CH₃COONa·3H₂O 640 mg/L, NH₄Cl 57 mg/L, K₂HPO₄·3H₂O 22 mg/L, CaCl₂ 11.5 mg/L, MgSO₄ 12 mg/L, and 10 mL of the trace element solution, which is similar to those used in previous studies [3], [9]. Both reactors were placed at room temperature (25±1°C) and sludge was not discharged during the operation.

At the end of the experimental period (75 days), biofilms were scraped from MBR_C anode (A_C), MBR_C cathode (C_C), MBR_O anode (A_O) and MBR_O cathode (C_O) to analyze the differences in the microbial communities using 454 pyrosequencing.

Analysis of the microbial communities

DNA extraction and PCR amplification.

DNA was extracted from the microbial communities in A_C, A_O, C_C and C_O according to methods described previously [10]. To amplify the 16S rRNA from the samples the following universal primers were used: 8F (5′-AGAGTTTGATCCTGGCTCAG-3′) and 533R (5′-TTACCGCGGCTGCTGGCAC-3′). Each PCR reaction was carried out in a 20 μL reaction volume containing 4 μL 5× FastPfu Buffer, 2 μL 2.5 mM dNTPs, 0.4 μL of each primer, 0.5 μL DNA and 0.4 μL FasrPfu Polymerase (TransStart FastPfu DNA Polymerase, TransGen, China). The thermocycling steps used for the PCR were: 95°C for 2 min, 25 cycles of 95°C for 30 sec followed by 55°C for 30 sec, and 72°C for 30 sec, and a final extension at 72°C for 5 min. After amplification, the amplicons were purified directly from the PRP mixture using the UNIQ-10 PCR purification Kit (Sangon, Shanghai, China) and quantified using TBS-380 (Turner BioSystems, Inc., USA).

454 pyrosequencing.

A mixture of the purified amplicons was used for 454 pyrosequencing on a Roche massively parallel 454 GS-FLX Titanium sequencer (Roche 454 Life Sciences, Branford, CT, USA). To improve the quality of pyrosequencing data, defective reads were removed from the libraries; these included reads without a recognizable reverse primer, reads shorter than 150 bp, and those containing any ambiguous base call [10]. Then barcodes and primers were trimmed from the resulting sequences. The final pyrosequencing data contained 6381 (A_O), 6854 (A_C), 12243 (C_O), 7097 (C_C) high quality V1–V3 tags for the 16S rRNA-gene. The raw reads were deposited into the NCBI Sequence Read Archive (SRA) database (Accession Number: SRA114114).

Classification of the microbial communities.

Pyrosequencing reads were clustered into operational taxonomic units (OTUs) with an average length of 390 bp. Then the OTUs were further clustered using the MOTHUR program (http://www.Mothur.org/wiki/Main-Page) with sequence distances set at 0.03 or 0.05. Based on these clusters the following parameters were calculated for each sample: Shannon diversity index (http://www.mothur.org/wiki/Shannon), Chao1 richness (http://www.mothur.org/wiki/Chao), abundance-based coverage using the abundance coverage estimator (ACE) (http://www.mothur.org/wiki/Ace), Good's coverage (http://www.mothur.org/wiki/Coverage), and the rarefaction curves at α 0.03 and 0.05. Based on MOTHUR and SILVA106 database, representative reads from the clusters were classified with a confidence threshold of 80% at the levels of both phyla and genera.

Results and Discussion

Performance of the bioelectrochemical MBRs

In the bioelectrochemical MBR under closed-circuit operation, the stainless-steel membrane module with biofilm formation not only serves as a biocathode for the MFC but also as a dynamic membrane for efficient solid/liquid separation [4]. In both MBR systems, effluent turbidity of 0.8 NTU (Nephelometric turbidity unit) was reached within 24 h. In addition, the average efficiencies of chemical oxygen demand (COD) and NH₄⁺-N removal during the operation were 86.1% and 97.5% for MBR_C, and 84.9% and 96.4% for MBR_O. Maximum power density of the MBR under closed-circuit operation was as high as 8.6 W/(m³ anode net volume), indicating that the biochemical MBR not only achieved efficient wastewater treatment but also power production [4]. Experimental results also demonstrated that the MFC (the anodic chamber under closed-circuit operation) could increase the degradation rate of organic matters by 7.0–13.0% compared with the anode chamber in the open-circuit mode, and the Coulombic efficiencies of the MFC under closed-circuit operation were 1.9%, 3.2%, 4.5% and 12.3% in the four runs, respectively [4].

Microbial richness and diversity

In our study, four 16S rDNA gene libraries were constructed by high-throughput sequencing of microbial communities from A_O, A_C, C_O and C_C samples. After trimming, sorting and quality control, 6381(A_O), 6854(A_C), 12243(C_O) and 7097(C_C) high-quality sequence tags (average length - 390 bp) were clustered into 1859 (A_O), 1488 (A_C), 1997 (C_O) and 1856 (C_C) operational taxonomic units (OTUs) at 3% distance thresholds, and 1602 (A_O), 1211 (A_C), 1583 (C_O) and 1493 (C_C) OTUs at 5% distance thresholds (Table 1). The abundance-based coverage estimator (ACE), Chao1, Shannon and Good Coverage are also presented in Table 1. Higher numbers of OTUs were estimated for A_O sample (4719 and 7816 in A_O, 3424 and 5712 in A_C, respectively) with infinite sampling at 3% distance by Chao1 estimator and ACE. This indicated that the richness of the bacterial communities in the MFC anode operated under open circuit was higher than that under closed circuit mode. However, for the cathode samples, microbial richness of Cc was greater than Co (Table 1). The Shannon diversity index values for A_O and C_C at 0.03/0.05 distance were higher than A_C and C_O, respectively, suggesting higher diversity in the microorganisms in A_O than A_C, while similar higher diversity was observed in C_C when compare to C_O. Since the anodes and cathodes of the two bioelectrochemical MBRs were initially inoculated with the same sludge, the observed differences in the microbial richness and diversity between the bioelectrodes could be attributed to power generation.

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Table 1. Similarity based OTUs and species richness estimates of the bacterial phylotypes in the four samples.

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The rarefaction curves of all four samples at 3% and 5% distance thresholds are shown in Fig. 2. Evidently none of the rarefaction curves reached a plateau in this study, and new OTUs continued to emerge even after 12000 reads were sampled with pyrosequencing. The results indicated that pyrosequencing could successfully reveal the higher diversity of bacterial communities in MFC compared to other conventional molecular biological methods, such as DGGE and clone library [11]–[13]. Different slopes observed in the rarefaction curves represented diversity of the samples, and steeper slopes such as in A_O indicated higher sample diversity when compared to A_C and C_C. Among all four samples C_O was the least diverse.

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Figure 2. Rarefaction curves based on 16S rDNA sequences of the bacterial communities from anode (A) and cathode (B) samples.

The OTUs are calculated based on 3% and 5% distances.

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Taxonomic complexity of the bacterial communities

Phylogenetic analysis was used to characterize the anode and cathode microbial community structure and composition in the MBRs under open and closed circuit modes. A comparison of the relative bacterial community abundance at the phylum level for the anode and cathode samples is shown in Fig. 3. The number of phyla present in the A_O and A_C samples was nearly identical except for the minor phyla (Deferribacteres and Gemmatimonadetes), which accounted for less than 0.1% of the total community in the A_O sample.

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Figure 3. Relative abundance of bacterial reads retrieved from the anodes (A) and cathodes (B) in the open and closed circuit MFC models (Phylum level).

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In the anode samples, 22 phyla were identified. Deferribacteres and Gemmatimonadetes were detected in A_O while they were not present in A_C. Among the total reads, 7.1% from A_O and 5.3% from A_C were not classified at the phylum level, indicating that at least some bacteria in the anode biofilms were not cultured. Proteobacteria and Bacteroidetes (45.2% and 15.5% for A_O; 55.0% and 14.8% for A_C) were the most abundant in both anode samples (Fig. 3), which is consistent with previous studies on MFCs anode biofilm analyzed by 454 pyrosequencing [14]–[16]. It should be noted that Proteobacteria was less abundant in A_O than in A_C, which could be associated with the differential abundance in Deltaproteobacteria (25.1% in A_O and 38.9% in A_C). The reason for this could be that some of the known exoelectrogenic bacteria (e.g., Desulfuromonas) belong to the phylum Deltaproteobacteria [17]. We also found that Chloroflexi (10.6%) was another major phylum represented in A_O sample. Previous studies had reported that the predominant bacteria in the anaerobic digester sludge was Chloroflexi [18], which is capable of assimilating N-acetyl-D-glucosamine, a major structural component in bacterial cells [19]. In the A_C sample, the third major phylum was Firmicutes (8.14%) besides the most abundant phyla Proteobacteria and Bacteroidetes. Previous studies have shown that Firmicutes was predominant in glucose-fed MFCs [16], [20], and the phylum could not be identified when MFC was switched to acetate-fed mode [20]. However, Firmicutes was detected in both anode samples in the present study, suggesting that Firmicutes could have originated from the inoculum and/or by symbiotic relationship among bacteria in the anodes. Moreover, Firmicutes was enriched in A_C than A_O, which could be related to its ability to transfer extracellular electrons and it is likely that the metabolites produced by Pseudomonas (also enriched in A_C) enabled Firmicutes (Gram-positive) to achieve this extracellular electron transfer function [21].

In the cathode samples, only 15 phyla were identified in total. Fibrobacteres were absent in C_O, while Armatimonadetes and Spirochaetes were not found in C_C. Only 1.08% of the total sequences in C_O and 1.06% in C_C were not identified at the phylum level, which were lesser than those in the anode samples. The dominant phyla were Proteobacteria (64.85% in C_O and 71.61% C_C) and Bacteroidetes (25.2% in Co and 19.2% in C_C) (Fig. 3), followed by Planctomycetes (4.75%) and Chloroflexi (1.45%) in C_O, and Planctomycetes (2.92%) and Chlorobi (1.70%) in C_C. Although the majority of phyla in both cathode samples were similar, C_O had abundant Bacteroidetes, while C_C had more Protebacteria, which comprised of Alphaproteobacteria (C_O - 5.7%, C_C - 15.3%), Betaproteobacteria (C_O - 49.2%, Cc - 45.3%), Deltaproteobacteria (C_O - 3.1%, Cc - 3.1%), Gammaproteobacteria (C_O - 6.1%, Cc - 6.4%), and Epsilonproteobacteria (C_O - 0.1%, Cc - 0.01%) classes. Betaproteobacteria is a well-known ammonia-oxidizing bacteria, and was discovered as a low abundant class in cathode biofilms from ammonia-lacking MFC [22], and the predominant class in ammonia-containing MFCs [14], [23]. The enrichment of Betaproteobacteria in both cathode samples was consistent with the high ammonia removal efficiency of MBR_C and MBR_O (97.5% and 96.4%). Further, Alphaproteobacteria was robust in C_C than C_O, suggesting that the cathode in the bioelectrochemical MBR under closed-circuit operation facilitated the growth of Alphaproteobacteria [24]. In comparison with traditional dynamic MBR, the microbial community compositions in the bioelectrochemical MBR are also different. For instance, Chlorobi, Chloroflexi and Planctomycetes with relative abundance >1% were detected in our system, while they were absent in the dynamic MBRs reported by others [25]. This might indicate that the bioelectrochemical MBR owns its special community possibly due to the power generation.

Changes in the microbial community in bioelectrochemical MBRs under open and closed circuit modes

To further elucidate the differences among microbial communities between the two systems, all four samples were compared at the genus level. Relative abundance (>0.5%) of the most dominant taxa in A_O and A_C is depicted in Fig. 4A. Interestingly, Desulfobacter, which has not been reported in any bioelectrochemical systems (BES) thus far, was the most abundant bacteria (16.6% in A_O and 15.0% in A_C) in the anodes. This could be attributed to the fact that the inoculum used in this study was collected from the anaerobic unit of an anaerobic/anoxic/oxic-MBR with a longer sludge retention time (SRT = 60 d) and indeed, Desulfobacter was reported previously in this MBR [26]. Although both systems had the same dominant genus (Desulfobacter), the microbial communities between the two anode samples were quite different at the genus level. The relative abundance of Desulfuromonas, which is a known electrogenic bacteria, was much higher in A_C (10.2%) when compared to A_O (0.11%). This indicated that the power generation impacts microbial metabolism and that closed-circuit operation acclimated more electrogenic bacteria.

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Figure 4. Relative abundance of the predominant groups in anode (A) and cathode (B) samples at the genus level.

Relative abundance is defined as the number of sequences affiliated to a particular taxon divided by the total number of sequences per sample (%). Genera with relative abundance less than 0.5% in both libraries are defined as “others”.

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Microbial groups with electrochemical activities were observed in the anodes (gray shaded region in Fig. 4A) and included Desulfobulbus, Desulfuromonas, Pseudomonas and Arcobacter (0.64%, 0.11%, 0.89% and 1.6% in A_O; 0.96%, 10.2%, 1.2% and 0.55% in A_C, respectively). Desulfobulbus is reported to not only use soluble electron-acceptors such as sulfate and Fe (III) but also uses the electrode surface as electron acceptor when pyruvate, lactate, propionate or hydrogen are provided as electron donors without exogenous electron-shuttling compounds for electricity production [27]. Desulfuromonas can also oxidize ethanol, propanol, and butanol with Fe (III) as electron acceptor [28]. However, Bond et al. reported that Desulfuromonas can conserve energy to support their growth by oxidizing organic compounds such as acetate and benzoate with an electrode acceptor [29]. Pseudomonas can produce a soluble redox metabolite, pyocyanin, which mediates the transfer of electrons between bacteria and the anode in an MFC [30]. Besides, Arcobacter can associate with the electrode and rapidly generate a strong electronegative potential in the presence of acetate [31]. In the present study, the high abundance of Desulfuromonas and low abundance of Desulfobulbus and Pseudomonas is likely due to the use of acetate as electron donor. However, Arcobacter, which uses acetate as the electron donor and an electrode as the electron acceptor, was abundant in A_O than A_C presumably due to the competition between Desulfuromonas and Arcobacter for the electron donor (acetate). In addition to these, A_C also contained some minor bacterial populations (relative abundance <1%) such as Clostridium, Comamonas and Geobacter all of which have the capacity to generate electricity [17].

Leptolinea and Longilinea were represented in larger fractions in A_O (2.1% and 2.0%) than in A_C (0.28% and 0.26%) (Fig. 4A), suggesting that these two genera might not grow well in the closed-circuit anode biofilm. Such limitation in Ac could be due to the fact that both are strict filamentous anaerobes used in fermenting carbohydrates, and are in general isolated from thermophilic or mesophilic sludge [32]. Notably, Rhodobacter, a well-known photofermentative bacteria that produces hydrogen from many organic substrates [33], [34] was enriched in A_C (1.61%) than A_O (0.55%). Previously, Rhodobacter was shown to be directly involved in power production [35].

Interestingly, the microbial community structure between C_O and C_C samples was very different (Fig. 4B). Sphaerotilus was the most dominant bacteria in both C_O and C_C samples with a relative abundance of 32.2% and 20.8% respectively, followed by Flexibacter (18.9%), and Dokdonella (4.2%) in C_O, and Flexibacter (11.7%), and Rhodobacter (9.3%) in C_C. Both Sphaerotilus and Flexibacter were the dominant genera shared by both C_O and C_C samples, and these genera have been reported to be frequently responsible for filamentous bulking in activated sludge [36], [37]. However, in Cc a decrease in their abundance demonstrated that the closed-circuit conditions can alleviate filamentous bulking of activated sludge. Rhodobacter, which is a hydrogen producing bacteria [33] and Hydrogenophaga, an autotrophic H₂-oxidizing bacteria that utilizes hydrogen as the energy source [38], were accumulated in the C_C biofilm (9.3% - Rhodobacter and 5.0% - Hydrogenophaga) (Fig. 4B). However, they only accounted for 3.2% and 2.6% in C_O, respectively. Thrash et al. demonstrated that microorganisms could accept electrons from a solid-state electrode via the cathodic production of hydrogen, which mediates the transfer of electrons [39]. Therefore, both Rhodobacter and Hydrogenophaga could be presumed to play a role in electron transfer from the cathode surface to the terminal electron acceptor.

Through 454 pyrosequencing, the functional microbes for bioelectricity generation are clarified. The present work also shows that the microbial community structure in the cathode is different. These results present the potential for further improving the system performance through regulation of electrogenic microbes as microorganisms play a key role in organic matter degradation and power generation. The enrichment of functional microbes for enhancing the power density needs further studying since now the optimization of the system mainly relies on reactor configuration, electrode materials and separators.

Conclusions

High-throughput 454 pyrosequencing revealed that the bioelectrochemical MBRs operated under open and closed circuit conditions could result in diverse microbial community structures. Chao1 estimators and Shannon diversity indexes indicated that the microorganisms in A_O was richer and highly diverse than those in A_C. However, among the cathodes C_C revealed a richer and more diverse microbial community when compared to C_O. The microbial community composition in the anode samples revealed that Proteobacteria and Bacteroidetes were the dominant phyla in Ao and Ac, while Firmicutes was enriched in A_C. Deltaproteobacteria affiliated to Proteobacteria were also more abundant in A_C than A_O. In addition, the relative abundance of Desulfuromonas, which are well-known electrogenic bacteria, was much higher in A_C compared to A_O, indicating that closed-circuit operation can acclimate more electrogenic bacteria. In the cathode samples, Protebacteria were robust in C_C while Bacteroidetes were more abundant in C_O. Rhodobacter and Hydrogenophaga were represented more in C_C than C_O, suggesting that the two genera could play a role in electron transfer from the surface of cathode to the terminal electron acceptors in the bioelectrochemical MBR under closed-circuit operation. Changes in the microbial community between the two bioelectrochemical MBRs demonstrated that the power generation affected the microbial community structure in both anode and cathode biofilms, facilitating the selection of functional microbes in the closed-circuit operation system for power generation.

Author Contributions

Conceived and designed the experiments: ZWW JH CWZ ZCW. Performed the experiments: JH XRZ. Analyzed the data: JH JXM ZWW. Contributed reagents/materials/analysis tools: CWZ ZCW JXM. Wrote the paper: JH ZWW.

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Figures

Abstract

Introduction

Materials and Methods

Experimental set-up

Inoculation and operation

Analysis of the microbial communities

DNA extraction and PCR amplification.

454 pyrosequencing.

Classification of the microbial communities.

Results and Discussion

Performance of the bioelectrochemical MBRs

Microbial richness and diversity

Taxonomic complexity of the bacterial communities

Changes in the microbial community in bioelectrochemical MBRs under open and closed circuit modes

Conclusions

Author Contributions

References