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Quantification of Hyphomicrobium Populations in Activated Sludge from an Industrial Wastewater Treatment System as Determined by 16S rRNA Analysis

机译:通过16S rRNA分析确定工业废水处理系统中活性污泥中的微量微生物数量

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摘要

The bacterial community structure of the activated sludge from a 25 million-gal-per-day industrial wastewater treatment plant was investigated using rRNA analysis. 16S ribosomal DNA (rDNA) libraries were created from three sludge samples taken on different dates. Partial rRNA gene sequences were obtained for 46 rDNA clones, and nearly complete 16S rRNA sequences were obtained for 18 clones. Seventeen of these clones were members of the beta subdivision, and their sequences showed high homology to sequences of known bacterial species as well as published 16S rDNA sequences from other activated sludge sources. Sixteen clones belonged to the alpha subdivision, 7 of which showed similarity to Hyphomicrobium species. This cluster was chosen for further studies due to earlier work on Hyphomicrobium sp. strain M3 isolated from this treatment plant. A nearly full-length 16S rDNA sequence was obtained from Hyphomicrobium sp. strain M3. Phylogenetic analysis revealed that Hyphomicrobium sp. strain M3 was 99% similar to Hyphomicrobium denitrificans DSM 1869T in Hyphomicrobium cluster II. Three of the cloned sequences from the activated sludge samples also grouped with those of Hyphomicrobium cluster II, with a 96% sequence similarity to that of Hyphomicrobium sp. strain M3. The other four cloned sequences from the activated sludge sample were more closely related to those of the Hyphomicrobium cluster I organisms (95 to 97% similarity). Whole-cell fluorescence hybridization of microorganisms in the activated sludge with genus-specific Hyphomicrobium probe S-G-Hypho-1241-a-A-19 enhanced the visualization of Hyphomicrobium and revealed that Hyphomicrobium appears to be abundant both on the outside of flocs and within the floc structure. Dot blot hybridization of activated sludge samples from 1995 with probes designed for Hyphomicrobium cluster I and Hyphomicrobium cluster II indicated that Hyphomicrobium cluster II-positive 16S rRNA dominated over Hyphomicrobium cluster I-positive 16S rRNA by 3- to 12-fold. Hyphomicrobium 16S rRNA comprised approximately 5% of the 16S rRNA in the activated sludge.
机译:使用rRNA分析研究了每天2500万加仑工业废水处理厂的活性污泥的细菌群落结构。从在不同日期采集的三个污泥样品创建了16S核糖体DNA(rDNA)库。对于46个rDNA克隆,获得了部分rRNA基因序列,对于18个克隆,获得了近乎完整的16S rRNA序列。这些克隆中有17个是β细分的成员,它们的序列与已知细菌物种的序列以及来自其他活性污泥来源的公开的16S rDNA序列具有高度同源性。 16个克隆属于alpha细分,其中7个与Hyphomicrobium物种相似。由于对Hyphomicrobium sp的早期研究,选择了该簇用于进一步研究。从该处理厂分离的菌株M3。从Hyphomicrobium sp。获得了几乎全长的16S rDNA序列。菌株M3。系统发育分析表明,Hyphomicrobium sp。 M3菌株与Hyphomicrobium cluster II中的Hyphomicrobium denitrificans DSM 1869 T 相似。从活性污泥样品中克隆的三个序列也与Hyphomicrobium cluster II的序列分组,与Hyphomicrobium sp的序列相似性为96%。菌株M3。来自活性污泥样品的其他四个克隆序列与Hyphomicrobium cluster I生物的相似性更高(95%到97%的相似性)。用属特异性的Hyphomicrobium探针SG-Hypho-1241-aA-19对活化污泥中的微生物进行全细胞荧光杂交,增强了Hyphomicrobium的可视性,并揭示了Hyphomicrobium在絮凝物的外部和絮凝结构中似乎都很丰富。 。 1995年活化污泥样品与针对Hyphomicrobium cluster I和Hyphomicrobium cluster II设计的探针的斑点印迹杂交表明,Hyphomicrobium cluster II阳性的16S rRNA相对Hyphomicrobium Cluster I阳性的16S rRNA占3至12倍。 Hyphomicrobium 16S rRNA约占活性污泥中16S rRNA的5%。

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