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通过原位杂交和微电极评估生物强化和生物刺激的影响。

Evaluation of the impact of bioaugmentation and biostimulation by in situ hybridization and microelectrode.

作者信息

Satoh Hisashi, Okabe Satoshi, Yamaguchi Yuki, Watanabe Yoshimasa

机构信息

Department of Environmental and Civil Engineering, Hachinohe Institute of Technology, Aomori 031-8501, Japan.

出版信息

Water Res. 2003 May;37(9):2206-16. doi: 10.1016/S0043-1354(02)00617-6.

Abstract

Three rotating disk biofilm reactors were operated to evaluate whether bioaugmentation and biostimulation can be used to improve the start-up of microbial nitrification. The first reactor was bioaugmented during start-up period with an enrichment culture of nitrifying bacteria, the second reactor received a synthetic medium containing NH(4)(+) and NO(2)(-) to facilitate concomitant proliferation of ammonia- and nitrite-oxidizing bacteria, and the third reactor was used as a control. To evaluate the effectiveness of bioaugmentation and biostimulation approaches, time-dependent developments of nitrifying bacterial community and in situ nitrifying activity in biofilms were monitored by fluorescence in situ hybridization (FISH) technique and microelectrode measurements of NH(4)(+), NO(2)(-), NO(3)(-), and O(2). In situ hybridization results revealed that addition of the enrichment culture of nitrifying bacteria significantly facilitated development of dense nitrifying bacterial populations in the biofilm shortly after, which led to a rapid start-up and enhancement of in situ nitrification activity. The inoculated bacteria could proliferate and/or survive in the biofilm. In addition, the addition of nitrifying bacteria increased the abundance of nitrifying bacteria in the surface of the biofilm, resulting in the higher nitrification rate. On the other hand, the addition of 2.1mM NO(2)(-) did not stimulate the growth of nitrite-oxidizing bacteria and did inhibit the proliferation of ammonia-oxidizing bacteria instead. Thus, the start-up of NO(2)(-) oxidation was unchanged, and the start-up of NH(4)(+) oxidation was delayed. In all the three biofilm reactors, data sets of time series analyses on population dynamics of nitrifying bacteria determined by FISH, in situ nitrifying activities determined by microelectrode measurements, and the reactor performances revealed an approximate agreement between the appearance of nitrifying bacteria and the initiation of nitrification activity, suggesting that the combination of these techniques was a very powerful monitoring tool to evaluate the effectiveness of bioaugmentation and biostimulation strategies.

摘要

运行了三个旋转盘式生物膜反应器,以评估生物强化和生物刺激是否可用于改善微生物硝化作用的启动。第一个反应器在启动期用硝化细菌富集培养物进行生物强化,第二个反应器接受含有NH(4)(+)和NO(2)(-)的合成培养基,以促进氨氧化细菌和亚硝酸盐氧化细菌的同步增殖,第三个反应器用作对照。为了评估生物强化和生物刺激方法的有效性,通过荧光原位杂交(FISH)技术以及对NH(4)(+)、NO(2)(-)、NO(3)(-)和O(2)的微电极测量,监测生物膜中硝化细菌群落随时间的发展以及原位硝化活性。原位杂交结果表明,添加硝化细菌富集培养物在不久后显著促进了生物膜中密集硝化细菌群体的发展,这导致原位硝化活性的快速启动和增强。接种的细菌能够在生物膜中增殖和/或存活。此外,添加硝化细菌增加了生物膜表面硝化细菌的丰度,从而导致更高的硝化速率。另一方面,添加2.1mM NO(2)(-)并未刺激亚硝酸盐氧化细菌的生长,反而抑制了氨氧化细菌的增殖。因此,NO(2)(-)氧化的启动没有变化,而NH(4)(+)氧化的启动被延迟。在所有三个生物膜反应器中,通过FISH确定的硝化细菌种群动态的时间序列分析数据集、通过微电极测量确定的原位硝化活性以及反应器性能表明,硝化细菌的出现与硝化活性的启动之间存在大致的一致性,这表明这些技术的组合是评估生物强化和生物刺激策略有效性的非常强大的监测工具。

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