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Subjects Waste Management and Disposal

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Waste Management and Disposal


Publications
37

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CitationNamesAbstract
High-temperature EBPR process: The performance, analysis of PAOs and GAOs and the fine-scale population study of Candidatus “Accumulibacter phosphatis” Ong et al. (2014). Water Research 64
Simple, rapid and effective preservation and reactivation of anaerobic ammonium oxidizing bacterium “Candidatus Brocadia sinica” Ali et al. (2014). Water Research 57 Ca. Brocadia sinica
Potential for Growth of Candidatus 'Accumulibacter phosphatis' in an Aerobic Shaking Culture Fukushima et al. (2010). Journal of Water and Environment Technology 8 (2)
Endogenous metabolism of Candidatus Accumulibacter phosphatis under various starvation conditions Lu et al. (2007). Water Research 41 (20) “Accumulibacter phosphatis”
Development of the Quantitative PCR Method for Candidatus ‘Accumulibacter phosphatis’ and Its Application to Activated Sludge Fukushima et al. (2007). Journal of Water and Environment Technology 5 (1)
Obtaining highly enriched cultures of Candidatus Accumulibacter phosphates through alternating carbon sources Lu et al. (2006). Water Research 40 (20) “Accumulibacter”
Comparison between Direct Microscopy and Flow Cytometry for rRNA‐Based Quantification of Candidatus Accumulibacter phosphatis in Activated Sludge Perez‐Feito et al. (2006). Water Environment Research 78 (2) “Accumulibacter phosphatis”
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Comparison between Direct Microscopy and Flow Cytometry for rRNA‐Based Quantification of Candidatus Accumulibacter phosphatis in Activated Sludge
A comparison of the quantification of a specific microbial group in activated sludge by fluorescent in‐situ hybridization, coupled with either direct microscopic counting or flow cytometry, was performed using an enhanced‐biological‐phosphorus‐removal, sequencing‐batch reactor. The population dynamics of Candidatus Accumulibacter phosphatis (Cand. A. phosphatis) was evaluated during two separate runs of the reactor. With the operational conditions used, Cand. A. phosphatis was enriched until a failure in the pH controller eliminated its ecological advantage. As a result, the comparison of quantification techniques included Cand. A. phosphatis concentrations as low as 11% and as high as 96% of the total cells in the samples. The analysis demonstrated that, regardless of the particular limitations of each technique, both provided similar results when the activated‐sludge flocs were easily dispersed. However, when the activated‐sludge samples contained flocs that were difficult to disperse, flow cytometry failed to provide quantitative results.
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