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首页> 外文期刊>Applied and Environmental Microbiology >In situ analysis of denitrifying toluene- and m-xylene-degrading bacteria in a diesel fuel-contaminated laboratory aquifer column.
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In situ analysis of denitrifying toluene- and m-xylene-degrading bacteria in a diesel fuel-contaminated laboratory aquifer column.

机译:在受柴油燃料污染的实验室含水层色谱柱中对甲苯和间二甲苯降解细菌的反硝化原位分析。

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摘要

A diesel fuel-contaminated aquifer was bioremediated in situ by the injection of oxidants (O2 and NO3-) and nutrients in order to stimulate microbial activity. After 3.5 years of remediation, an aquifer sample was excavated and the material was used (i) to isolate bacterial strains able to grow on selected hydrocarbons under denitrifying conditions and (ii) to construct a laboratory aquifer column in order to simulate the aerobic and denitrifying remediation processes. Five bacterial strains isolated from the aquifer sample were able to grow on toluene (strains T2 to T4, T6, and T10), and nine bacterial strains grew on toluene and m-xylene (strains M3 to M7 and M9 to M12). Strains T2 to T4, T6, and T10 were cocci, and strains M3 to M7 and M9 to M12 were rods. The morphological and physiological differences were also reflected in small sequence variabilities in domain III of the 23S rRNA and in the 16S rRNA. Comparative sequence analyses of the 16S rRNA of one isolate (T3 and M3) of each group revealed a close phylogenetic relationship for both groups of isolates to organisms of the genus Azoarcus. Two 16S rRNA-targeted oligonucleotide probes (Azo644 and Azo1251) targeting the experimental isolates, bacteria of the Azoarcus tolulyticus group, and Azoarcus evansii were used to investigate the significance of hydrocarbon-degrading Azoarcus spp. in the laboratory aquifer column. The number of bacteria in the column determined after DAPI (4',6-diamidino-2-phenylindole) staining was 5.8 x 10(8) to 1.1 x 10(9) cells g of aquifer material-1. About 1% (in the anaerobic zone of the column) to 2% (in the aerobic zone of the column) of these bacteria were detectable by using a combination of probes Azo644 and Azo1251, demonstrating that hydrocarbon-degrading Azoarcus spp. are significant members of the indigenous microbiota. More than 90% of the total number of bacteria were detectable by using probes targeting higher phylogenetic groups. Approximately 80% of these bacteria belonged to the beta subdivision of the class Proteobacteria (beta-Proteobacteria), and 10 to 16% belonged to the gamma-Proteobacteria. Bacteria of the alpha-Proteobacteria were present in high numbers (10%) only in the aerobic zone of the column.
机译:通过注入氧化剂(O2和NO3-)和养分,对受柴油燃料污染的含水层进行原位生物修复,以刺激微生物活动。经过3.5年的修复,挖掘出一个含水层样品,并使用该材料(i)分离能够在反硝化条件下在选定的碳氢化合物上生长的细菌菌株,以及(ii)构建实验室的含水层柱,以模拟好氧和反硝化作用。修复过程。从含水层样品中分离出的五个细菌菌株能够在甲苯上生长(菌株T2至T4,T6和T10),九个细菌菌株在甲苯和间二甲苯上生长(菌株M3至M7和M9至M12)。菌株T2至T4,T6和T10为球菌,菌株M3至M7和M9至M12为棒。形态和生理学差异也反映在23S rRNA结构域III和16S rRNA结构域的小序列变异中。每组一个分离株(T3和M3)的16S rRNA的比较序列分析表明,这两组分离株与固氮菌属生物有密切的系统发育关系。使用两个靶向16S rRNA的寡核苷酸探针(Azo644和Azo1251)靶向实验分离株,甲苯佐假单胞菌(Azoarcus tolulyticus)组的细菌和埃文氏假单胞菌(Azoarcus evansii),以研究降解烃的拟南芥的重要性。在实验室含水层柱中。 DAPI(4',6-diamidino-2-phenylindole)染色后确定的柱中细菌数为5.8 x 10(8)至1.1 x 10(9)g含水层材料-1。通过使用探针Azo644和Azo1251的组合,可检测到大约1%(在色谱柱的厌氧区)至2%(在色谱柱的需氧区),这证明了降解烃的Azoarcus spp。是土著微生物群的重要成员。通过使用针对较高系统发育群体的探针,可检测到细菌总数的90%以上。这些细菌中约80%属于变形杆菌类(β-Proteobacteria)的β细分,而10至16%则属于γ-变形杆菌。 α-变形杆菌的细菌仅在色谱柱的需氧区中大量存在(10%)。

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