4.6 Article

Thermophilic Alkaline Fermentation Followed by Mesophilic Anaerobic Digestion for Efficient Hydrogen and Methane Production from Waste-Activated Sludge: Dynamics of Bacterial Pathogens as Revealed by the Combination of Metagenomic and Quantitative PCR Analyses

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出版社

AMER SOC MICROBIOLOGY
DOI: 10.1128/AEM.02632-17

关键词

waste-activated sludge; thermophilic alkaline fermentation; mesophilic anaerobic digestion; bacterial pathogens; metagenomic analysis; qPCR analysis

资金

  1. National Key Research and Development Program of China [2015BAD15B06, 2017YFC0212205]
  2. National Natural Science Foundation of China [51408133, 51750110498]
  3. State Key Laboratory of Pollution Control and Resource Reuse Foundation [PCRRF16009]
  4. Science and Technology Commission of Shanghai Municipality [17230740900]

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Thermophilic alkaline fermentation followed by mesophilic anaerobic digestion (TM) for hydrogen and methane production from waste-activated sludge (WAS) was investigated. The TM process was also compared to a process with mesophilic alkaline fermentation followed by a mesophilic anaerobic digestion (MM) and one-stage mesophilic anaerobic digestion (M) process. The results showed that both hydrogen yield (74.5 ml H-2/g volatile solids [VS]) and methane yield (150.7 ml CH4/g VS) in the TM process were higher than those (6.7 ml H-2/g VS and 127.8 ml CH4/g VS, respectively) in the MM process. The lowest methane yield (101.2 ml CH4/g VS) was obtained with the M process. Taxonomic results obtained from metagenomic analysis showed that different microbial community compositions were established in the hydrogen reactors of the TM and MM processes, which also significantly changed the microbial community compositions in the following methane reactors compared to that with the M process. The dynamics of bacterial pathogens were also evaluated. For the TM process, the reduced diversity and total abundance of bacterial pathogens in WAS were observed in the hydrogen reactor and were further reduced in the methane reactor, as revealed by metagenomic analysis. The results also showed not all bacterial pathogens were reduced in the reactors. For example, Collinsella aerofaciens was enriched in the hydrogen reactor, which was also confirmed by quantitative PCR (qPCR) analysis. The study further showed that qPCR was more sensitive for detecting bacterial pathogens than metagenomic analysis. Although there were some differences in the relative abundances of bacterial pathogens calculated by metagenomic and qPCR approaches, both approaches demonstrated that the TM process was more efficient for the removal of bacterial pathogens than the MM and M processes. IMPORTANCE This study developed an efficient process for bioenergy (H-2 and CH4) production from WAS and elucidates the dynamics of bacterial pathogens in the process, which is important for the utilization and safe application of WAS. The study also made an attempt to combine metagenomic and qPCR analyses to reveal the dynamics of bacterial pathogens in anaerobic processes, which could overcome the limitations of each method and provide new insights regarding bacterial pathogens in environmental samples.

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