Abstract
Mixed microbial cultures have become a preferred choice of biocatalyst for chain elongation systems due to their ability to convert complex substrates into medium-chain carboxylates. However, the complexity of the effects of process parameters on the microbial metabolic networks is a drawback that makes the task of optimizing product selectivity challenging. Here, we studied the effects of small air contaminations on the microbial community dynamics and the product formation in anaerobic bioreactors fed with lactate, acetate and H2/CO2. Two stirred tank reactors and two bubble column reactors were operated with H2/CO2 gas recirculation for 139 and 116 days, respectively, at pH 6.0 and 32°C with a hydraulic retention time of 14 days. One reactor of each type had periods with air contamination (between 97 ± 28 and 474 ± 33 mL O2 L−1 d−1, lasting from 4 to 32 days), while the control reactors were kept anoxic. During air contamination, production of n-caproate and CH4 was strongly inhibited, whereas no clear effect on n-butyrate production was observed. In a period with detectable O2 concentrations that went up to 18%, facultative anaerobes of the genus Rummeliibacillus became predominant and only n-butyrate was produced. However, at low air contamination rates and with O2 below the detection level, Coriobacteriia and Actinobacteria gained a competitive advantage over Clostridia and Methanobacteria, and propionate production rates increased to 0.8–1.8 mmol L−1 d−1 depending on the reactor (control reactors 0.1–0.8 mmol L−1 d−1). Moreover, i-butyrate production was observed, but only when Methanobacteria abundances were low and, consequently, H2 availability was high. After air contamination stopped completely, production of n-caproate and CH4 recovered, with n-caproate production rates of 1.4–1.8 mmol L−1 d−1 (control 0.7–2.1 mmol L−1 d−1). The results underline the importance of keeping strictly anaerobic conditions in fermenters when consistent n-caproate production is the goal. Beyond that, micro-aeration should be further tested as a controllable process parameter to shape the reactor microbiome. When odd-chain carboxylates are desired, further studies can develop strategies for their targeted production by applying micro-aerobic conditions.
Highlights
Anaerobic fermentation with mixed microbial communities is an appealing option for the production of medium-chain carboxylates (MCCs) (De Groof et al, 2019)
With the help of gas recirculation systems, this study aimed to investigate the effects of small air contamination on the dynamics of the microbial community and the product formation in MCCproducing fermenters
bubble column reactors (BCRs) were assembled and operated with the following differences in relation to the stirred tank reactors (STRs): 1) the BCR vessels consisted of bubble columns made of glass with a working volume of 1.2 L each; 2) the systems had no oxidation-reduction potential (ORP) monitoring; 3) pH monitoring and correction was done manually three times a week; 4) temperature regulation was carried out via the water jacket of the vessels and a thermal bath; 5) gas recirculation was carried out with micro-diaphragm gas pumps NMP 830 (KNF Neuberger GmbH, Freiburg, Germany) at a flow of ca. 1.5 L min−1; and 6) an internal vertical hollow glass with holes of 1–2 mm was used to bubble the gas into the broth
Summary
Anaerobic fermentation with mixed microbial communities is an appealing option for the production of medium-chain carboxylates (MCCs) (De Groof et al, 2019). Almost all isolated MCC producers are strict anaerobes (one exception was described by Stamatopoulou et al (2020)) to which O2 causes damage via direct and indirect ways. O2 gives rise to reactive oxygen species (ROS), such as O2− and H2O2, which are intermediates produced during O2 reduction that severely damage cells if not promptly neutralized (Johnson and Hug, 2019). Even though every cultured microorganism has mechanisms to deal with ROS (Johnson and Hug, 2019), obligate anaerobic bacteria such as Clostridium spp. suffer from O2 due to their high dependence on O2-sensitive enzymes (e.g., ferredoxin-dependent oxidoreductases or [FeFe]-hydrogenases) (Imlay, 2006; Khademian and Imlay, 2020). Exposure to O2 causes some hydrogenases to decompose or to form additional ROS that damage other parts of the cell (Stiebritz and Reiher, 2012)
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