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Efficient Metabolic Exchange and Electron Transfer within a Syntrophic Trichloroethene-Degrading Coculture of Dehalococcoides mccartyi 195 and Syntrophomonas wolfei

机译:代谢降解三氯乙烯的共代Dehalococcoides mccartyi 195和Syntrophomonas wolfei内的高效代谢交换和电子转移

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Dehalococcoides mccartyi 195 (strain 195) and Syntrophomonas wolfei were grown in a sustainable syntrophic coculture using butyrate as an electron donor and carbon source and trichloroethene (TCE) as an electron acceptor. The maximum dechlorination rate (9.9 ± 0.1 μmol day?1) and cell yield [(1.1 ± 0.3) × 108 cells μmol?1 Cl?] of strain 195 maintained in coculture were, respectively, 2.6 and 1.6 times higher than those measured in the pure culture. The strain 195 cell concentration was about 16 times higher than that of S. wolfei in the coculture. Aqueous H2 concentrations ranged from 24 to 180 nM during dechlorination and increased to 350 ± 20 nM when TCE was depleted, resulting in cessation of butyrate fermentation by S. wolfei with a theoretical Gibbs free energy of ?13.7 ± 0.2 kJ mol?1. Carbon monoxide in the coculture was around 0.06 μmol per bottle, which was lower than that observed for strain 195 in isolation. The minimum H2 threshold value for TCE dechlorination by strain 195 in the coculture was 0.6 ± 0.1 nM. Cell aggregates during syntrophic growth were observed by scanning electron microscopy. The interspecies distances to achieve H2 fluxes required to support the measured dechlorination rates were predicted using Fick's law and demonstrated the need for aggregation. Filamentous appendages and extracellular polymeric substance (EPS)-like structures were present in the intercellular spaces. The transcriptome of strain 195 during exponential growth in the coculture indicated increased ATP-binding cassette transporter activities compared to the pure culture, while the membrane-bound energy metabolism related genes were expressed at stable levels.
机译:使用丁酸盐作为电子供体,碳源和三氯乙烯(TCE)作为电子受体,在可持续的共生共培养中生长了Dehalococcoides mccartyi 195(株195)和Syntrophomonas wolfei。在共培养中维持的菌株195的最大脱氯速率(9.9±0.1μmol·day?1)和细胞产量[(1.1±0.3)×108细胞μmol?1 Cl?]分别是在联合培养中测得的2.6和1.6倍。纯文化。在共培养中,菌株195的细胞浓度比沃尔夫链霉菌高约16倍。在脱氯过程中,H2水溶液的H2浓度范围为24至180 nM,当TCE耗尽时,H2的浓度增加至350±20 nM,导致沃尔夫链球菌停止丁酸盐发酵,理论吉布斯自由能为?13.7±0.2 kJ mol?1。共培养物中的一氧化碳约为每瓶0.06μmol,低于隔离菌株195中观察到的一氧化碳。共培养中菌株195对TCE脱氯的最小H2阈值为0.6±0.1 nM。通过扫描电子显微镜观察到在营养生长期间的细胞聚集。使用菲克定律预测了达到支持测得的脱氯速率所需的H2通量的种间距离,并证明了聚集的必要性。在细胞间隙存在丝状附肢和细胞外聚合物(EPS)样结构。与纯培养物相比,在共培养物中指数生长期间菌株195的转录组表明ATP结合盒转运蛋白活性增加,而膜结合的能量代谢相关基因以稳定水平表达。

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