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Journal ArticleDOI

Identification of acetate- or methanol-assimilating bacteria under nitrate-reducing conditions by stable-isotope probing.

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TLDR
It is analyzed how growth of bacterial populations was stimulated by acetate or methanol as the external carbon source in nitrogen-removal systems and characterized nitrite reductase genes (nirS and nirK) as functional marker genes for denitrifier communities in acetate- or meethanol-assimilating populations.
Abstract
Stable-isotope probing (SIP) was used to identify acetate- or methanol-assimilating bacteria under nitrate-reducing conditions in activated sludge. A sludge sample obtained from wastewater treatment systems was incubated in a denitrifying batch reactor fed with synthetic wastewater containing [13C]acetate or [13C]methanol as the main carbon source and nitrate as the electron acceptor. We analyzed how growth of bacterial populations was stimulated by acetate or methanol as the external carbon source in nitrogen-removal systems. Most of the acetate- or methanol-assimilating bacteria identified by SIP have been known as denitrifiers in wastewater treatment systems. When acetate was used as the carbon source, 16S rRNA gene sequences retrieved from 13C-labeled DNA were closely related to the 16S rRNA genes of Comamonadaceae (e.g., Comamonas and Acidovorax) and Rhodocyclaceae (e.g., Thauera and Dechloromonas) of the Betaproteobacteria, and Rhodobacteraceae (e.g., Paracoccus and Rhodobacter) of the Alphaproteobacteria. When methanol was used as the carbon source, 16S rRNA gene sequences retrieved from 13C-DNA were affiliated with Methylophilaceae (e.g., Methylophilus, Methylobacillus, and Aminomonas) and Hyphomicrobiaceae. Rarefaction curves for clones retrieved from 13C-DNA showed that the diversity levels for methanol-assimilating bacteria were considerably lower than those for acetate-assimilating bacteria. Furthermore, we characterized nitrite reductase genes (nirS and nirK) as functional marker genes for denitrifier communities in acetate- or methanol-assimilating populations and detected the nirS or nirK sequence related to that of some known pure cultures, such as Alcaligenes, Hyphomicrobium, and Thauera. However, most of the nirS or nirK sequences retrieved from 13C-DNA were clustered in some unidentified groups. On the basis of 16S rRNA gene clone libraries retrieved from 13C-DNA, these unidentified nir sequences might be identified by examining the nir gene in candidates for true denitrifiers (e.g., the families Comamonadaceae, Hyphomicrobiaceae, Methylophilaceae, and Rhodobacteraceae).

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Journal ArticleDOI

DNA stable-isotope probing

TL;DR: General guidelines for incubating environmental samples with labeled substrate are highlighted and a detailed protocol for separating labeled DNA from unlabeled community DNA is provided, which maximizes the recovery oflabel DNA from CsCl gradients.
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Microbial ecology of denitrification in biological wastewater treatment.

TL;DR: This review stresses the need to integrate microbial ecology information into conventional denitrification design and operation at full-scale, and a combination of high-throughput approaches is next in line for thorough assessment of wastewater denitrifying community structure and function.
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Performance and Microbial Community Analysis of a Novel DEAMOX Based on Partial-Denitrification and Anammox Treating Ammonia and Nitrate Wastewaters

TL;DR: High-throughput sequencing analysis revealed that Thauera genera were dominant in both SBRs and possibly played a key role for partial-denitrification with high NO2--N accumulation and the Denitratisoma capable of complete denitrification (NO3--N→N2) was found in R2 that might lead to lower NTR.
Journal ArticleDOI

A conceptual ecosystem model of microbial communities in enhanced biological phosphorus removal plants

TL;DR: The EBPR process is a perfect model system for studies of microbial ecology in water engineering systems and this conceptual model can be used for proposing and testing theories based on microbial ecosystem theories, for the development of new and improved quantitative ecosystem models and is beneficial for future design and management of wastewater treatment systems.
Journal ArticleDOI

Who eats what, where and when? Isotope-labelling experiments are coming of age.

TL;DR: Some of the most recent isotope techniques reviewed, with an emphasis on methodological improvements to the sensitivity and utility of these methods, hold promise to transform the way the authors link phylogeny and function in complex microbial communities.
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Journal ArticleDOI

Cell biology and molecular basis of denitrification.

TL;DR: Denitrification is intimately related to fundamental cellular processes that include primary and secondary transport, protein translocation, cytochrome c biogenesis, anaerobic gene regulation, metalloprotein assembly, and the biosynthesis of the cofactors molybdopterin and heme D1.
Journal ArticleDOI

Stable-isotope probing as a tool in microbial ecology

TL;DR: Stable-isotope probing offers a powerful new technique for identifying microorganisms that are actively involved in specific metabolic processes under conditions which approach those occurring in situ.
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