An Outbreak of Nonflocculating Catabolic Populations Caused the Breakdown of a Phenol-Digesting Activated-Sludge Process

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Applied and Environmental Microbiology, July 1999, p. 2813-2819, Vol. 65, No. 7
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

An Outbreak of Nonflocculating Catabolic Populations Caused the Breakdown of a Phenol-Digesting Activated-Sludge Process

Kazuya Watanabe,^* Maki Teramoto, and Shigeaki Harayama

Marine Biotechnology Institute, Kamaishi Laboratories, Heita, Kamaishi City, Iwate, Japan

Received 1 February 1999/Accepted 13 April 1999

Activated sludge was fed phenol as the sole carbon source, and the phenol-loading rate was increased stepwise from 0.5 to1.0 g liter¹ day¹ and then to 1.5 g liter¹ day¹. After the loading rate was increased to 1.5 g liter¹ day¹, nonflocculating bacteria outgrew the sludge, and the activated-sludgeprocess broke down within 1 week. The bacterial population structureof the activated sludge was analyzed by temperature gradient gelelectrophoresis (TGGE) of PCR-amplified 16S ribosomal DNA (rDNA)fragments. We found that the population diversity decreased asthe phenol-loading rate increased and that two populations (designatedpopulations R6 and R10) predominated in the sludge during thelast several days before breakdown. The R6 population was presentunder the low-phenol-loading-rate conditions, while the R10 populationwas present only after the loading rate was increased to 1.5 gliter¹ day¹. A total of 41 bacterial strains with different repetitive extragenicpalindromic sequence PCR patterns were isolated from the activatedsludge under different phenol-loading conditions, and the 16SrDNA and gyrB fragments of these strains were PCR amplified andsequenced. Some bacterial isolates could be associated with majorTGGE bands by comparing the 16S rDNA sequences. All of the bacterialstrains affiliated with the R6 population had almost identical16S rDNA sequences, while the gyrB phylogenetic analysis dividedthese strains into two physiologically divergent groups; bothof these groups of strains could grow on phenol, while one group(designated the R6F group) flocculated in laboratory media andthe other group (the R6T group) did not. A competitive PCR analysisin which specific gyrB sequences were used as the primers showedthat a population shift from R6F to R6T occurred following theincrease in the phenol-loading rate to 1.5 g liter¹ day¹. The R10 population corresponded to nonflocculating phenol-degradingbacteria. Our results suggest that an outbreak of nonflocculatingcatabolic populations caused the breakdown of the activated-sludgeprocess. This study also demonstrated the usefulness of gyrB-targetedfine population analyses in microbialecology.

^* Corresponding author. Mailing address: Marine Biotechnology Institute, Kamaishi Laboratories, 3-75-1 Heita, Kamaishi City,Iwate 026-0001, Japan. Phone: 81 193 26 6537. Fax: 81 193 26 6584.E-mail: kazwata{at}kamaishi.mbio.co.jp.

Applied and Environmental Microbiology, July 1999, p. 2813-2819, Vol. 65, No. 7
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

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