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Investigation of an Acetate-Fed Denitrifying Microbial Community by Stable Isotope Probing, Full-Cycle rRNA Analysis, and Fluorescent In Situ Hybridization-Microautoradiography

机译:醋酸同位素反硝化微生物群落的稳定同位素探测,全周期rRNA分析和荧光原位杂交-微放射自显影技术研究。

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摘要

The acetate-utilizing microbial consortium in a full-scale activated sludge process was investigated without prior enrichment using stable isotope probing (SIP). [13C]acetate was used in SIP to label the DNA of the denitrifiers. The [13C]DNA fraction that was extracted was subjected to a full-cycle rRNA analysis. The dominant 16S rRNA gene phylotypes in the 13C library were closely related to the bacterial families Comamonadaceae and Rhodocyclaceae in the class Betaproteobacteria. Seven oligonucleotide probes for use in fluorescent in situ hybridization (FISH) were designed to specifically target these clones. Application of these probes to the sludge of a continuously fed denitrifying sequencing batch reactor (CFDSBR) operated for 16 days revealed that there was a significant positive correlation between the CFDSBR denitrification rate and the relative abundance of all probe-targeted bacteria in the CFDSBR community. FISH-microautoradiography demonstrated that the DEN581 and DEN124 probe-targeted cells that dominated the CFDSBR were capable of taking up [14C]acetate under anoxic conditions. Initially, DEN444 and DEN1454 probe-targeted bacteria also dominated the CFDSBR biomass, but eventually DEN581 and DEN124 probe-targeted bacteria were the dominant bacterial groups. All probe-targeted bacteria assessed in this study were denitrifiers capable of utilizing acetate as a source of carbon. The rapid increase in the number of organisms positively correlated with the immediate increase in denitrification rates observed by plant operators when acetate is used as an external source of carbon to enhance denitrification. We suggest that the impact of bacteria on activated sludge subjected to intermittent acetate supplementation should be assessed prior to the widespread use of acetate in the wastewater industry to enhance denitrification.
机译:在没有事先浓缩的情况下,使用稳定同位素探测(SIP)对全规模活性污泥工艺中利用乙酸盐的微生物财团进行了研究。在SIP中使用[13C]乙酸酯标记反硝化剂的DNA。对提取的[13C] DNA馏分进行全周期rRNA分析。 13C文库中的优势16S rRNA基因系统型与Betaproteobacteria类中的Comamonadaceae和Rhodocyclaceae细菌家族密切相关。设计了七种用于荧光原位杂交(FISH)的寡核苷酸探针以特异性靶向这些克隆。将这些探针应用于连续进料的反硝化测序间歇反应器(CFDSBR)运行16天的污泥中发现,CFDSBR的反硝化率与CFDSBR社区中所有以探针为目标的细菌的相对丰度之间存在显着的正相关。 FISH显微放射自显影显示,在CFDSBR中占主导地位的DEN581和DEN124探针靶向细胞能够在缺氧条件下摄取[14C]乙酸盐。最初,针对DEN444和DEN1454探针的细菌也主导了CFDSBR生物量,但是最终,针对DEN581和DEN124探针的细菌成为了主要细菌群。在这项研究中评估的所有以探针为目标的细菌都是能够利用乙酸盐作为碳源的反硝化剂。当乙酸盐用作外部碳源以增强反硝化作用时,生物体数量的快速增加与工厂经营者观察到的反硝化率立即增加呈正相关。我们建议,在废水工业中广泛使用乙酸盐以增强反硝化作用之前,应先评估细菌对醋酸盐间歇性补充的活性污泥的影响。

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