Nitrogen Cycling and Community Structure of Proteobacterial beta -Subgroup Ammonia-Oxidizing Bacteria within Polluted Marine Fish Farm Sediments

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Applied and Environmental Microbiology, January 1999, p. 213-220, Vol. 65, No. 1
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Nitrogen Cycling and Community Structure of Proteobacterial $beta$ -Subgroup Ammonia-Oxidizing Bacteria within Polluted Marine Fish Farm Sediments

Allison E. McCaig,¹ Carol J. Phillips,²^,³ John R. Stephen,¹^,⁴^, George A. Kowalchuk,⁵ S. Martyn Harvey,² Rodney A. Herbert,³ T. Martin Embley,⁴ and James I. Prosser¹^,^*

Department of Molecular and Cell Biology, Institute of Medical Sciences, University of Aberdeen, Foresterhill, Aberdeen AB25 2ZD,¹ Dunstaffnage Marine Laboratory, Oban, Argyll PA34 4AD,² and Department of Biological Sciences, University of Dundee, Dundee DD1 4HN,³ Scotland, and Department of Zoology, The Natural History Museum, London SW7 5BD, England,⁴ United Kingdom, and Department of Plant Microorganism Interactions, Netherlands Institute of Ecology, 6666 ZG Heteren, The Netherlands⁵

Received 22 June 1998/Accepted 20 October 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

A multidisciplinary approach was used to study the effects of pollution from a marine fish farm on nitrification rates andon the community structure of ammonia-oxidizing bacteria in theunderlying sediment. Organic content, ammonium concentrations,nitrification rates, and ammonia oxidizer most-probable-numbercounts were determined in samples of sediment collected from beneatha fish cage and on a transect at 20 and 40 m from the cage. Thedata suggest that nitrogen cycling was significantly disrupteddirectly beneath the fish cage, with inhibition of nitrificationand denitrification. Although visual examination indicated someslight changes in sediment appearance at 20 m, all other measurementswere similar to those obtained at 40 m, where the sediment wasconsidered pristine. The community structures of proteobacterial $beta$ -subgroup ammonia-oxidizing bacteria at the sampling sites werecompared by PCR amplification of 16S ribosomal DNA (rDNA), usingprimers which target this group. PCR products were analyzed bydenaturing gradient gel electrophoresis (DGGE) and with oligonucleotidehybridization probes specific for different ammonia oxidizers.A DGGE doublet observed in PCR products from the highly pollutedfish cage sediment sample was present at a lower intensity inthe 20-m sample but was absent from the pristine 40-m sample station.Band migration, hybridization, and sequencing demonstrated thatthe doublet corresponded to a marine Nitrosomonas group whichwas originally observed in 16S rDNA clone libraries prepared fromthe same sediment samples but with different PCR primers. Ourdata suggest that this novel Nitrosomonas subgroup was selectedfor within polluted fish farm sediments and that the relativeabundance of this group was influenced by the extent ofpollution.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

In recent years, the culture of Atlantic salmon (Salmo salar L.) has become of major industrial importance worldwide, leadingto concern over the impact of fish farming on previously pristinemarine environments. Intensive cage cultivation of fish leadsto localized pollution of the adjacent seabed through accumulationof uneaten food and fecal material (14, 21). The impact ofthis organic enrichment on the underlying sediment is affectedby several factors, such as water currents, turbulence, and depthand the duration, quality, and quantity of waste loading (41),and anaerobic conditions can develop, resulting in the outgassingof hydrogen sulfide, ammonia, andmethane.

The major component of fish feed is protein, and the output from fish farms, therefore, has a high nitrogen content. Thismay lead to eutrophication, since nitrogen is the major nutrientlimiting phytoplankton growth (9). Nitrification, the oxidationof ammonia to nitrate via nitrite, is central to the cycling ofnitrogen in the environment and, when coupled with denitrification,alleviates the effects of eutrophication through removal of nitrogento the atmosphere as nitrous oxide or dinitrogen gas (5). Nitrification,however, is sensitive to low oxygen tension, sulfur compounds,high ammonia and nitrite concentrations, and the presence of abroad range of organic compounds (3, 20, 22, 24). Insituations of chronic pollution, nitrification and, consequently,the coupled process of denitrification are often completely suppressed,exacerbating the environmental impact of the aquaculture industry(21).

The ammonia-oxidizing bacteria carry out the first, rate-limiting stage of nitrification, the conversion of ammonia to nitrite.The intractability of these organisms to isolation and laboratorycultivation has, until recently, prevented meaningful study oftheir community structure and diversity in natural environments.Phylogenetic analysis of pure cultures, based on 16S rRNA sequencedata, has demonstrated that the ammonia-oxidizing bacteria canbe divided into two groups. The first contains Nitrosococcus oceanusand forms a deep branch within the $gamma$ subgroup of the class Proteobacteria(44). The second group, containing the majority of culturedstrains, forms a tight cluster within the $beta$ -subgroup proteobacteriaand can be subdivided into two clades, corresponding to Nitrosomonasspp. and Nitrosospira spp. (12, 43). Sequence analysis ofpartial 16S ribosomal DNA (rDNA) clones (1,099 bases) obtainedfrom marine sediment and soil samples by using primers specificfor the $beta$ -subgroup ammonia oxidizers (27) revealed that theenvironmental sequences which have been isolated so far from marinesediments and from soil form at least six clusters, four withinthe Nitrosospira clade and two within the Nitrosomonas clade (Fig.1) (37). Stephen et al. (37) also presented the first evidencefor the existence of marine representatives of the genus Nitrosospira.Analysis of alignments of shorter rDNAs, which included sequencesfrom marine enrichment cultures, indicated that a seventh group,associated with Nitrosomonas europaea and Nitrosomonas eutropha,may also exist (37). Pure-culture representatives have now beenisolated for all groups (40, 42) with the exception of Nitrosospiracluster 1 and Nitrosomonas cluster 5, although sequences fromthese two groups have been amplified from enrichment culturesof ammonia-oxidizing bacteria (37).

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FIG. 1. Neighbor-joining tree showing the relationship of the single sequence obtained from two excised DGGE gel bands, designated DGGE (1 & 2), to environmental sequences and reference $beta$ -subgroup proteobacteria based on analysis of 424 bases of aligned 16S rDNA sequences. The percentages of bootstrap support above 50% are shown for distance matrix analysis at nodes concerning major ammonia oxidizer relationships. Clusters (Cl.) 1 to 7 are indicated. Clone sequences obtained from sediment DNA libraries are prefixed Env. EnvA clones were obtained from polluted sediment beneath the fish cage, while EnvB and EnvC clones were obtained at distances of 20 and 40 m, respectively. Other environmental clone sequences (prefixed pH) and the enrichment sequence Enrich ZD5 were isolated from soil. For convenience, the tree has been pruned from a larger tree containing additional sequences from reference proteobacteria. The scale is 1% estimated change. For the design of the oligonucleotide probe, it was necessary to subdivide cluster 6, indicated by the asterisk, into two groups. Cluster 6a, represented by pH4.2A/23 on this tree, comprises a small cluster of three soil clones. All other known sequences belonging to cluster 6 are designated cluster 6b.

rRNA sequence analysis has been used to compare ammonia oxidizer populations within acid and neutral soils and in fish farmsediments with various degrees of organic pollution (37). Asmall group of novel Nitrosomonas sequences, designated cluster5, was detected within polluted sediments but not within a pristinesediment, suggesting that nitrogen-rich organic pollution fromfish farming may be selecting for or providing a source of particularammonia oxidizers. Denaturing gradient gel electrophoresis (DGGE)(29) provides an alternative approach to the analysis of rDNAclone libraries and has recently been used successfully to demonstratedifferences in ammonia oxidizer populations in sand dune sites(23). PCR amplification products are electrophoresed througha denaturing polyacrylamide gel, enabling investigation of populationdifferences through the presence or absence of bands in environmentalsamples. Bands can then be identified by using a range of oligonucleotideprobes with various specificities within the $beta$ -subgroup ammoniaoxidizers (38). This approach has been used to confirm selectionfor particular ammonia oxidizers within acid- and neutral-pH agriculturalsoils (38).

The aim of this study was to investigate the effects of organic particulate material from a marine fish farm on the ammoniaoxidizer community structure in the underlying sediment by using16S rDNA-based techniques and to relate these effects to processmeasurements. Furthermore, because the same DNA extracts wereused in this study and in that of Stephen et al. (37), it waspossible to compare inferred population structures by using twodifferent primer sets and different analyticalmethods.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Fish farm location and cage history. The fish farm used in this study consisted of two sets of six cages and a fallow site situated in Glenmore Bay, Loch Sunart,West Scotland, United Kingdom (Ordnance Survey Map coordinate592 618) at a water depth of 16 m. Samples were collected fromcages which had been stocked with Atlantic salmon (Salmo salarL.) for 11 months following a 4-month fallowperiod.

Sample collection. Sediment samples (eight cores per sampling station) were collected in Perspex core tubes (59-mm inner diameter by 300-mm length)by divers at four stations. Station A was situated directly underneatha fish cage, while stations B and C were located on a transectleading from the cage, at distances of 20 and 40 m, respectively.An additional sample, from a transect at a distance of 10 m fromthe cage (station S), was also collected for chemical analysis,rate measurements, and cell counts only. Cores were transportedto the laboratory in insulated boxes and stored at 8 to 10°C inthe dark until processed (within 12h).

After preliminary visual macroscopic inspection of the core appearance, the top 0.5 cm of each core was aseptically removedfor analysis. Duplicate cores from stations A, B, and C were usedin molecular analyses. After removal of subsamples of sedimentfor enrichment of marine ammonia-oxidizing bacteria (describedin reference 37), samples (approximately 1 g each) were storedin sterile Eppendorf tubes at $-$ 70°C prior to DNA extraction. Fornutrient determination, rate measurements, and most-probable-number(MPN) bacterial counts, two sets of three sediment cores (i.e.,six cores) from stations A to C and station S were pooled to providetwo replicates per samplingpoint.

Organic-matter content, porosity, and water content. To determine the porosity and water content of sediments, six 5-ml subsamples were taken by using disposable syringes withthe luer ends removed, and wet weight was determined in preweighedglass vials. Sediment samples were frozen and lyophilized to aconstant weight to give sediment dry-weight values, and the watercontent and porosity of each of the sediments were calculated.The organic-matter content of sediment was determined as weightloss by ignition (500°C, 12 h) of freeze-dried samples (approximately1 g each) (7).

Pore water nutrients. Concentrations of ammonia and nitrate in pore water were determined for each station. The pore water was separated from sedimentby centrifugation in a polypropylene tube at 2,000 × g for 10min. Supernatants were removed, filtered through Whatman GF/Ffilters in an N₂ atmosphere, and stored frozen until chemicalanalysis wasperformed.

Ammonia and nitrite oxidation rates. Ammonia and nitrite oxidation rates for each station were determined by a modification of the method of Bianchi et al. (4).For each replicate sediment sample, three subsamples (5 ml each)were deposited into each of three glass vials containing 10 mlof filtered (Whatman GF/F) seawater. One vial from each set wasused as a control (i.e., no additions). Allylthiourea and sodiumchlorate (final concentrations, 10 mg liter¹ and 10 mM, respectively) were added to the second and third vialsto inhibit ammonia and nitrite oxidation, respectively. Vialswere placed in a shaking water bath at 4°C, and nitrite concentrationswere determined for samples taken at 0, 4, 8, and 24h.

Ammonia, nitrite, and nitrate analyses. Samples were analyzed for ammonium and nitrate by the use of a Technicon II Automated Analyzer. Nitrite was measured by ascaled-down modification of the method of Parsons et al. (30).Samples (1 ml each) were pipetted into acid-washed 75- by 10-mmborosilicate glass test tubes, and 40 µl of sulfanilamide solution(0.01% [wt/vol] in 8.5 M hydrochloric acid) was added to each.The tube contents were vortexed and then incubated for 2 min,and 40 µl of n-(1-naphthyl)-ethylenediamine dihydrochloride (0.001%[wt/vol] in double-distilled water) was added to each. Tube contentswere vortexed and allowed to stand for 30 min, and absorbancereadings were obtained spectrophotometrically in 1-cm-light-pathcells at 543nm.

Denitrification rates. Rates of denitrification were determined by a modification of the method of Raymond et al. (31). Subsamples (2 ml) of eachreplicate sediment core were transferred into four 10-ml bottles,each containing 2 ml of seawater. The bottles were flushed withchemically pure nitrogen (grade CP; BOC, Guildford, United Kingdom)and sealed with butyl rubber stoppers. Reduction of N₂O to N₂was inhibited by addition of acetylene (15 kPa; BOC)-saturatedseawater (0.4 ml) to each bottle with a hypodermic syringe, andthe bottles were incubated at 20°C. Samples were taken at 0, 30,60, and 120 min by vortexing vigorously for 1 min before removalof 2.7 ml of the headspace into a preevacuated Monovette tube(Sarstedt Ltd., Leicester, United Kingdom). N₂O was detected witha Varian model 3400 gas chromatograph equipped with an electroncapture detector. Measured N₂O values were read against a standardcurve prepared with N₂O from Distillers MG Limited (Reigate, Surrey,UnitedKingdom).

Enumeration of nitrifying and nitrate-respiring bacteria. Ammonia oxidizers, nitrite oxidizers, and nitrate-respiring bacteria within sediment samples were enumerated by the MPN techniquein microtiter plates (32). This involved vigorously shakinga 1-ml sediment sample in 9 ml of sterile seawater containingapproximately 10 sterile glass beads (3 mm in diameter) for 1min. For each group of bacteria, 0.2 ml of the appropriate autoclavedmedium was dispensed into each well of a 96-well microtiter plate,and eight replicate twofold serial dilutions of sediment slurry(0.2 ml) were performed. Following incubation, wells were assayedfor the presence of each group of bacteria as described below,and numbers were calculated by using MPN tables (32).

Ammonia-oxidizing bacteria were enumerated in modified Watson's medium (16) prepared in artificial seawater, with the pHof the medium being adjusted to 7.5 by addition of sterile 5%Na₂CO₃ after autoclaving (121°C for 15 min). The pH indicatorphenol red was included in the medium to allow detection of areduction in pH below 7. Inoculated MPN plates were incubatedin the dark for 21 days at room temperature. Wells were scoredas positive for ammonia oxidizers by acid production and by detectionof NO₂ and NO₃ through development of a blue color after addition of 1 or 2drops of 0.2% (wt/vol) diphenylamine in concentrated H₂SO₄.

Nitrite-oxidizing bacteria were enumerated in the medium of Alexander and Clark (2) prepared in artificial seawater. Wellswere scored as positive for growth when nitrite was absent, asindicated by the lack of a color change upon addition of GriessIlosvay reagents 1 and2.

Nitrate respirers, i.e., those organisms capable of causing an increase in pH through reduction of nitrate to ammonia (dissimilatorynitrate reduction) or to nitrous oxide and nitrogen (denitrification),were enumerated in Alexander's (1) medium containing bromophenolblue as a pH indicator, which changes in color from yellow toblue with an increase in pH. Inoculated microtiter plates wereplaced in an anaerobic jar, the jar was sealed and then flushedwith oxygen-free nitrogen, and the plates were read after incubationin the dark for 7days.

DGGE. DNA was extracted directly from duplicate sediment samples from stations A, B, and C by a bead beating method (37). PCRamplification of a 498-bp PCR product and subsequent DGGE analysiswere carried out as described previously (23), using the primersCTO178f-GC and CTO637r. This primer pair was designed for specificamplification of a 460-bp region of the 16S rDNA of ammonia-oxidizingbacteria belonging to the proteobacterial $beta$ -subgroup and incorporationof a 38-bp GC clamp (35). PCR products were visualized by standardagarose electrophoresis followed by ethidium bromide staining.Approximately 200 ng of each product, estimated by visual referenceto molecular weight standards, was used in the subsequent DGGEanalysis. PCR amplification and DGGE analysis were also performedwith rDNA clones which represented each currently recognized clusterof marine $beta$ -subgroup ammonia oxidizers (37), as follows: EnvC1-17(Nitrosomonas cluster 6b), EnvB2-11 (Nitrosospira cluster 1),and EnvA1-21 (Nitrosomonas cluster 5). Polyacrylamide gels werestained with ethidium bromide and washed twice for 10 min eachin 0.5× TAE buffer (48.22 g of Tris base, 2.05 g of anhydroussodium acetate, and 1.86 g of Na₂EDTA · 2H₂O [pH 8] in 1 literof distilled water), and the UV gel image was then captured byusing the Imager system (Ampligene, Illkirch, France). DNA wastransferred to a nylon hybridization membrane, and the blot washybridized with $gamma$ -³²P-end-labelled oligonucleotide probes (listed in Table 1) bythe procedure of Stephen et al. (38). The identities of bandsfor clusters 1 and 6b were confirmed in this way. Bands correspondingto cluster 5 sequences were identified by comparison of theirmigration profiles with those of control clones and by sequenceanalysis of excised bands (described below). This was achievedby densitometry. The autoradiograph obtained by probing with $beta$ -AO233was scanned by using a model GS-700 imaging densitometer (Bio-Rad).For each lane on the gel, bands corresponding to each clusterwere selected and the data were processed by using the volumeanalysis function of Molecular Analyst software (version 1.5;Bio-Rad) and correcting for background signal. The relative abundanceof the three detected clusters in the environmental samples wascalculated as the percentage contribution of bands from each clusterto the total hybridization signal within each lane. Data are expressedas the means of duplicate samples.

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TABLE 1. Oligonucleotide probes and hybridization temperatures used in analysis of DGGE banding patterns of PCR-amplified rDNA of $beta$ -subgroup ammonia-oxidizing bacteria from polluted and pristine marine sediments

Recovery and sequence analysis of bands from the DGGE gel. The putative cluster 5 bands, which could not be identified by specific oligonucleotide hybridization, were excised from theDGGE gel, reamplified, and sequenced (23). Sequences were alignedagainst representative prokaryote 16S rRNA sequences from theRibosomal Database Project (26) and ammonia oxidizer sequences(27, 37). Sequence data were manipulated by using GeneticData Environment (GDE) software, version 2.2, distributed by theRibosomal Database Project. The GDE mask function was used toexclude from this analysis missing data or positions which couldnot be unambiguously aligned. Distance matrix analysis was performedby the Jukes and Cantor (19) correction and the neighbor-joiningmethod (33) implemented in PHYLIP 3.5 (10) operated throughGDEsoftware.

Nucleotide sequence accession numbers. The sequences of the upper and lower cluster 5 DGGE bands have been deposited in GenBank under accession no. AF006666 andAF006667.

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Macroscopic appearance of sediment samples. Core samples collected beneath the fish cage (station A) were extremely flocculant to a depth of 300 mm and consisted mostlyof decomposing fish feed and feces. Sulfide-oxidizing bacteriaformed a confluent white mat over the sediment surface, whilethe subsurface sediment was black due to the formation of ferroussulfide. At station S, the sediment was coarser in texture butwas otherwise similar to that at station A. At 20 m (station B),some signs of impaction were still apparent, although the ferroussulfide layer penetrated to a depth of only 10 mm. It should benoted, however, that the region of the cores analyzed in thisstudy (i.e., the top 0.5 cm) did not extend into the unaffectedsediment layers. At station C, 40 m from the fish cage, therewas no visual evidence of organicenrichment.

Organic content, water content, and sediment porosity. Organic content was highest directly beneath the fish cage, reflecting the high sedimentation rate of organic material, andwas significantly reduced (P < 0.05) at all other stations (Table2). Porosity and water content values of polluted sediments (0and 10 m) were high, as indicated by their more viscous nature,particularly at station A (0.88). All three parameters decreasedwith distance from the fish cage, and readings at the 40-m sitewere indicative of a tightly packed, pristine sediment, in contrastto the highly disturbed, liquefied surface of cores collectedfrom station A.

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TABLE 2. Water content, porosity, and organic matter content of sediments sampled directly beneath and on a transect extending from an Atlantic salmon farm cage

Ammonium, nitrate, and nitrous oxide concentrations. Ammonium levels directly beneath the fish cage were high (8 mmol liter¹) (Fig. 2), reflecting the nitrogen content of sedimenting detritus,and decreased dramatically with increasing distance from the cage.A similar profile was observed for sediment-bound ammonium (datanot shown). Pore water nitrite concentrations, although considerablylower than ammonium levels, were elevated directly beneath thecage while showing little variation over the remainder of thetransect (Fig. 2). Nitrous oxide (determined during time zerosampling of denitrification assays) was also detected, with concentrationsdecreasing with distance from the cage site (Fig. 2).

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FIG. 2. Changes in pore water ammonium (in millimoles per liter), nitrate, and nitrous oxide (both in micromoles per liter) concentrations in the 0- to 5-mm-depth-horizon sediment samples with increasing distance from the fish cage. Error bars represent standard errors for duplicate measurements.

Nitrification and denitrification rates. Ammonia and nitrite oxidation rates at increasing distances from the fish cage are shown in Fig. 3. At station A, directlybeneath the fish cage, rates for both ammonia and nitrite oxidationwere low (0.11 and 0.04 mmol of N m² day¹, respectively). At 10 m, ammonia and nitrite oxidation rateshad increased considerably, with similar values being observedat stations B and C. Denitrification, measured as accumulationof N₂O in the presence of acetylene, was not detected at any ofthe sampling points (data not shown).

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FIG. 3. Ammonia and nitrite oxidation rates (in millimoles per square meter per day) in the 0- to 5-mm-depth-horizon sediment samples with increasing distance from the fish cage. Error bars represent standard errors for duplicate measurements.

Enumeration of ammonia- and nitrite-oxidizing and nitrate-respiring bacteria. Numbers of ammonia-oxidizing bacteria were low at all stations and were generally only slightly above the lower detectionlimit (0.07 × 10⁶ bacteria m²) (Fig. 4). Despite the high concentration of ammonium at stationA, there was no increase in the number of ammonia oxidizers, consistentwith the low rates of ammonia oxidation measured at this station.A significant increase in numbers at station S was followed bya decrease over the remainder of the transect. A substantial populationof nitrite-oxidizing bacteria was detected at station A, directlybeneath the fish cage. The numbers decreased to detection levelby 10 m and did not vary greatly over the remainder of the transect.MPN counts of nitrate-respiring bacteria were highest at stationS, decreasing with distance from the cage.

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FIG. 4. MPN counts of ammonia and nitrite oxidizers and denitrifying bacteria in the 0- to 5-mm-depth-horizon sediment samples with increasing distance from the fish cage. Error bars represent standard errors for duplicate measurements.

DGGE analysis and oligonucleotide probing. PCR amplification products, with an incorporated GC clamp for DGGE analysis, were obtained for all six samples. Figure 5 illustratesthe ethidium bromide-stained polyacrylamide gel and autoradiographsobtained by the use of oligonucleotide probes specific for $beta$ -subgroupammonia oxidizers (Table 1).

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FIG. 5. DGGE analysis and Southern oligonucleotide hybridization following PCR amplification of $beta$ -subgroup ammonia-oxidizing bacteria from 0- to 5-mm-depth-horizon sediment samples obtained directly beneath the fish cage (0 m) and at distances of 20 and 40 m. Lanes 1 to 6, duplicate samples from stations A (lanes 1 and 2), B (lanes 3 and 4), and C (lanes 5 and 6); lane 7, EnvC1-17 (Nitrosomonas cluster 6b); lane 8, EnvB2-11 (Nitrosospira cluster 1); lane 9, EnvA1-21 (Nitrosomonas cluster 5). (A) An ethidium bromide-stained DGGE gel. (B to E) Oligonucleotide hybridizations. (B) Probe 1 (all $beta$ -subgroup ammonia oxidizers); (C) probe 2 (Nitrosospira cluster 1); (D) probe 3 (Nitrosomonas cluster 6b); (E) probe 4 (Nitrosomonas clusters 5, 6a, 6b, and 7).

Southern hybridization with probe $beta$ -AMO233 (Fig. 5B), designed for detection of all proteobacterial $beta$ -subgroup ammonia oxidizers,resulted in binding to all bands present on the ethidium bromide-stainedgel (Fig. 5A). The blots in Fig. 5C and D, probed with a cluster1 marine Nitrosospira-specific oligonucleotide and a probe formarine Nitrosomonas spp. (cluster 6b only), respectively, demonstratedthat these organisms were present in all sediment samples. Inthe blot shown in Fig. 5E, which illustrates the result of hybridizationwith a probe specific for all Nitrosomonas clusters (clusters5 to 7), an additional band doublet was detected, with an intensesignal in those lanes corresponding to highly polluted sediment(lanes 1 and 2), a less-intense signal at the 20-m station (lanes3 and 4), and no signal at 40 m (lanes 5 and 6). While the intensityof this doublet decreased with decreasing pollutant levels, thereappeared to be a corresponding increase in band intensity of thelower cluster 1 Nitrosospira sequences at the 20- and 40-m stations.This was confirmed by quantification of band densities (Fig. 6),which illustrates the relative signal contribution of bands fromeach subgroup to the total hybridization signal, estimated withthe $beta$ -AO233 probe, within DGGE products obtained at each samplingstation. The band doublets did not hybridize with either cluster6b (Fig. 5D)- or cluster 7 (data not shown)-specific oligonucleotideprobes but comigrated with the control clone for the novel, marineNitrosomonas clones. On the basis of current sequence information,it is not possible to design cluster 5-specific oligonucleotideprobes; hence, the identity was confirmed by sequence analysisof upper and lower bands. Both bands produced identical 422-bpsequences, and, as predicted, it appears that the degeneracy ofthe reverse PCR primer is responsible for the observed doubleteffect (23). A similar explanation may apply to the multiplebanding observed for the cluster 1 control. The cluster 5 DGGEsequences show >99% identity (1 bp mismatch) with the partialclone sequence EnvA2-13, obtained from the same sampling siteby using different PCR primers. Phylogenetic analysis illustratesclearly that these DGGE band sequences cluster within Nitrosomonascluster 5 (100% of bootstrapped replicates), as shown in Fig.1.

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FIG. 6. Relative abundance of $beta$ -subgroup ammonia-oxidizing bacteria from 0- to 5-mm-depth-horizon sediment samples obtained directly beneath the fish cage (0 m) and at distances of 20 and 40 m. Ammonia oxidizer clusters were resolved by DGGE, and relative band intensities were quantified by densitometry after probing with $beta$ -AMO233, which is specific for all $beta$ -subgroup ammonia-oxidizing bacteria. Error bars represent standard errors for duplicate sediment samples.

Quantification of the relative abundance of different clusters was carried out by densitometry. Figure 6 indicates the relativeband intensities obtained when probe $beta$ -AO223, which detects allclusters of proteobacterial $beta$ -subgroup ammonia oxidizers, wasused. Nitrosospira cluster 1 is the most abundant group at allthree sites, comprising 53 to 83% of the total signal in eachlane. This is in agreement with the original finding of Stephenet al. (37) that cluster 1 Nitrosospira spp. are found, andare potentially abundant, in marine environments. The relativequantity of signal from the cluster 5 bands, determined by usingthe $beta$ -AO223 probe (Fig. 5B), was significantly higher at siteA than at site B or C (P < 0.01). Similarly, the signal from siteB was significantly higher than that at site C (P < 0.01). Althoughin Fig. 5B to E there appears to be an increase in both clusters1 and 6 with increasing distance from the fish cage, no significantdifferences in the relative abundances of these groups at anyof the sites were observed. Quantification of the total signalfor each lane on the ethidium bromide-stained gel, and after probingwith $beta$ -AO233, indicates an increase in probe hybridization withdistance from the fish cage, despite approximately equal DNA loadings(data not shown). This may be explained by amplification of nontargetsequences during the PCR or the presence within polluted sedimentsof ammonia oxidizers with rDNA sequences which are not complementaryto oligonucleotides used in this study. Quantification of therelative abundance of Nitrosomonas clusters 5 and 6, when probedwith the Nitrosomonas probe Nmo254, confirms that the cluster5 signal significantly decreased, relative to the total signalwithin each lane, with increasing distance from the fish cage(data not shown). It was not possible in this study, however,to compare quantification of the relative abundance of cluster5 by using both the Nitrosomonas probe Nmo254 and $beta$ -AMO233. Along exposure of the autoradiograph for Nmo254 (Fig. 5E) was necessaryto visualize cluster 5 bands in lanes representing station B samples,but this resulted in saturation of cluster 5 and 6 controls, thuspreventing normalization of the data for the two probes. However,comparison of the ratios of each cluster within the environmentalsamples, using both probes, indicates that the probing efficienciesof the two oligonucleotides weresimilar.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

The aim of this study was to investigate the relationship between biological and chemical data on nitrogen cycling and communitystructure of proteobacterial $beta$ -subgroup ammonia-oxidizing bacteriain polluted and unpolluted sediments, combining traditional andmolecular biology-based methods. In addition, 16S rDNA sequenceanalysis (37) and DGGE analysis were compared by analyzing ammoniaoxidizers from the same sediment samples with specific PCR primerstargeted to different parts of the 16S rRNA gene. Only membersof the $beta$ -subgroup ammonia oxidizers were targeted for molecularanalysis, and $gamma$ -subgroup ammonia oxidizers and unknown nitrifyingorganisms may have a role in nitrogen flux within polluted andunpollutedsediments.

Chemical and biological analyses indicated that nitrogen cycling beneath the fish cage had been severely disrupted by sedimentationof nitrogen-rich organic material from the cage. This detritusaccumulation led to the formation of anaerobic sediment withinthe vicinity of the cage and undetectable levels of nitrificationand denitrification. This is consistent with studies of modelsystems artificially enriched with organic material (8, 36)and other fish farm locations (11, 21). It is possible thatnitrification was inhibited by the low oxygen penetration, whichgenerally decreases from 2 to 6 mm, in normal sediments, to lessthan 1 mm in areas of high organic loading (8, 18).

The largest populations of ammonia-oxidizing bacteria and the highest nitrification rates were observed at station S, 10 mfrom the fish cage, while lower but detectable levels of bothwere observed at the 20- and 40-m stations. From these data itcan be concluded that organic deposition from the fish cage didnot affect process measurements for nitrification at a distanceof 20 m, and the relative stimulation of ammonia oxidation atstation S can be explained by the presence of elevated, but noninhibitory,concentrations of ammonium and organic material. Molecular analysis,however, did indicate differences in the compositions of the ammoniaoxidizer communities directly beneath the fish cage and at 20m, as shown by the presence of novel sequences within clone libraries(37) and the detection of additional DGGE bands. The MPN methodfor enumeration of ammonia oxidizers indicated that populationsof less than 7 × 10⁴ bacteria m² (5-mm sampling depth) were present in the sediment underlyingthe fish cage, since no growth was shown in any replicates atany dilution factor tested. Stephen et al. (37), however, enrichedammonia-oxidizing bacteria from all of the same sediment samplesby using longer incubation periods. The appearance of novel bandsin those samples from polluted sites suggests that the changesin environmental conditions in the vicinity of the fish cage ledto selection for particular ammonia-oxidizing bacteria throughthe growth of these organisms and/or a decline of other membersof the community. The relative importance of each of these factorsis unknown, although pure-culture studies indicate that ammoniaoxidizer cell numbers remain stable throughout a range of environmentalstresses (15, 17).

Cell concentrations of ammonia and nitrite oxidizers and nitrification rates over the sampling transect were not closely correlated.It is highly likely that the standard culture conditions usedfor enumeration were not suitable for growth of all sediment ammoniaoxidizers, particularly since a single ammonium concentrationwas used in the growth medium while significantly different levelswere measured in the sediment samples at each station. In addition,it is possible that inhibitory substances present at the highlypolluted site adversely affected enumeration. Stephen et al. (37)demonstrated a bias toward Nitrosomonas spp. in enrichment culturesfrom the same sediment samples, while Nitrosospira spp. were moreabundant within clone libraries, suggesting that only a proportionof the total population will be enumerated. Similarly, the standardlaboratory conditions used for process measurements may have beensuboptimal for measurement of nitrification and denitrificationin the sediments obtained during this study. For example, thechlorate method for measurement of nitrification may have beenadversely affected within the polluted samples via inhibitionof ammonia oxidation through reduction of chlorate to chloriteby nitrite oxidizers (13). The application of ¹⁵N-based techniques might have provided more-accurate flux databut would have required considerably largersamples.

Although nitrification and denitrification were not detected, nitrous oxide production was measured at the fish cage siteand could have resulted from internal cycling of nitrogen withinan oxygen gradient. Ammonia and nitrite oxidation may have occurredwithin aerobic regions, providing substrate for the reductionof nitrate to ammonium, via nitrite and nitrous oxide, withinanaerobic regions. The resulting accumulation of nitrate and nitrousoxide beneath the fish cage may, therefore, have occurred becauseof an imbalance in the flux of nitrogen transformations withinthe system due to the particularly high levels of ammonium, i.e.,higher rates of ammonia oxidation than of ammonium recycling.It is also possible that nitrous oxide was produced as a by-productof ammonia oxidation, while Schmidt and Bock (34) recently demonstratedsimultaneous nitrification and denitrification by Nitrosomonaseutropha. Reduction of nitrate to ammonium may have been carriedout by the nitrite-oxidizing bacteria (28, 39) rather thanby heterotrophic nitrate-respiring bacteria. This is supportedby high MPN counts for nitrite oxidizers and detection of onlysmall populations of nitrate respirers at the polluted station.In a similar study, Kaspar et al. (21) showed that potentialdenitrification in sediment core slices collected from beneatha salmon fish cage was undetectable to a depth of 6 cm, whileother studies have demonstrated that ammonium recycling is favoredover denitrification when nitrate levels are low and the levelof organic matter is high (25).

In this study, DGGE analysis demonstrated a significant change in the community structure of ammonia oxidizers, the appearanceof a novel subgroup of Nitrosomonas spp., within the polluted-sedimentsamples, confirming preliminary results based on sequence analysisof 16S rDNA gene libraries of ammonia oxidizers prepared fromthe same sediment samples with different PCR primers. These strainsmay have increased tolerance to low oxygen tensions, to increasedammonium concentrations, or to the presence of inhibitory substancesor may have been introduced from external sources, such as fishfeed or fecal pellets. Cluster 5 sequences showing 98.5 to 99.5%sequence similarity to near-full-length (1.1-kb) cluster 5 sequencesfrom the polluted sediments have also been detected in an unpolluted,seaward sand dune site (23). Information on the relative abundanceof this novel subgroup in the sand dune site is not available,but in contrast to the polluted sediments, the nitrogen contentof the sand dune site was low. The physiological and environmentalsignificance of this group, therefore, remains unclear in theabsence of physiological analysis of pure-culturerepresentatives.

The presence of cluster 5 Nitrosomonas-like ammonia oxidizer strains within sediment collected at the 20-m site (Fig. 5A and5E) corresponds with visual observations of minimal organic impactat this site but not with any chemical indication of nitrogencycling disruption. This suggests that the community structureof the $beta$ -subgroup ammonia oxidizers is more sensitive to environmentalchanges than the physiological process carried out by these organisms,although it is important to note that community structure wasassessed by rDNA analysis alone in the present study. Since nitrificationwas also detected at the 10-m distance, it can be concluded thatthe detrimental impact of pollution from the fish farm was limitedto sediments in the immediate vicinity of the fishcage.

In conclusion, this study demonstrates clearly that DGGE analysis, in combination with Southern hybridization, representsan extremely elegant ecological tool for the analysis of bacterialdiversity and is particularly applicable to the investigationof proteobacterial $beta$ -subgroup ammonia oxidizers, a phylogeneticallyand physiologically constrained group of microorganisms. DGGEis a relatively inexpensive and rapid method of assessing populationdiversity, and while this technology cannot supersede sequenceanalysis, which is comparatively expensive, repetitive, and time-consuming,it has been shown to complement analysis of rDNA clone libraries.In this investigation, it was possible to link gross process andbiological measurements with more-subtle variation detected inthe community structure. Inclusion of data from a broad rangeof environmental parameters $---$ physical, chemical, and biological $---$ provedinvaluable in the interpretation of results from the molecularanalyses, highlighting the necessity for comprehensive, multidisciplinaryapproaches to the study of microbial ecology. This study has confirmedthe selection of a novel group of $beta$ -subgroup ammonia-oxidizingbacteria in sediments underlying and in proximity to fish farmcages. Further analysis of this group is necessary to understandfully its physiological and ecological significance in naturalenvironments.

	ACKNOWLEDGMENTS

We thank the Coastal Impact Research Group at Dunstaffnage Marine Laboratory (Oban, United Kingdom) for collection of thesamples.

This work was funded by NERC grant GST/02/568 to J.I.P. and T.M.E. as part of the NERC GAMES initiative and by MAFF grantAE 0511 to S.M.H.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular and Cell Biology, Institute of Medical Sciences, Universityof Aberdeen, Foresterhill, Aberdeen AB25 2ZD, Scotland, UnitedKingdom. Phone: 44 1224 273148. Fax: 44 1224 273144. E-mail: j.prosser{at}abdn.ac.uk.

Present address: Center for Environmental Biotechnology, University of Tennessee, Knoxville, TN 37932-2575.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

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1.	Alexander, M. 1965. Denitrifying bacteria, p. 1484-1486. In C. A. Black (ed.), Methods of soil analysis, vol. 9. American Society of Agronomy, Madison, Wis.
2.	Alexander, M., and F. E. Clark. 1965. Nitrifying bacteria, p. 1477-1483. In C. A. Black (ed.), Methods of soil analysis, vol. 9. American Society of Agronomy, Madison, Wis.
3.	Bédard, C., and R. Knowles. 1989. Physiology, biochemistry, and specific inhibitors of CH₄, NH₄⁺, and CO oxidation by methanotrophs and nitrifiers. Microbiol. Rev. 53:68-84[Abstract/Free Full Text].
4.	Bianchi, M., P. Bonin, and F. Feliatra. 1994. Bacterial nitrification and denitrification rates in the Rhone River plume (northwestern Mediterranean Sea). Mar. Ecol. Prog. Ser. 103:197-202.
5.	Blackburn, T. H., and N. D. Blackburn. 1992. Model of nitrification and denitrification in marine sediments. FEMS Microbiol. Lett. 100:517-522.
6.	Brosius, J., T. L. Dull, D. D. Sleeter, and H. F. Noller. 1981. Gene organisation and primary structure of a ribosomal RNA operon from Escherichia coli. J. Mol. Biol. 14:107-127.
7.	Byers, S. C., E. L. Mills, and P. L. Stewart. 1978. Measurements of the physical and chemical environments, p. 30-58. In N. A. Holme, and A. D. McIntyre (ed.), Methods for the study of marine benthos. Blackwell Scientific, Oxford, United Kingdom.
8.	Caffrey, J. M., N. P. Sloth, H. F. Kaspar, and T. H. Blackburn. 1993. Effect of organic loading on nitrification and denitrification in a marine sediment microcosm. FEMS Microbiol. Ecol. 12:159-167.
9.	Dugdale, R. C. 1967. Nutrient limitation in the sea: dynamics, identification and significance. Limnol. Oceanogr. 12:685-695.
10.	Felsenstein, J. 1993. PHYLIP: phylogeny inference package. University of Washington, Seattle.
11.	Hall, P. O. J., O. Holby, S. Kollberg, and M.-O. Samuelsson. 1992. Chemical fluxes and mass balances in a marine fish cage farm. IV. Nitrogen. Mar. Ecol. Prog. Ser. 89:81-91.
12.	Head, I. M., W. D. Hiorns, T. M. Embley, A. J. McCarthy, and J. R. Saunders. 1993. The phylogeny of autotrophic ammonia-oxidizing bacteria as determined by analysis of 16S ribosomal RNA gene sequences. J. Gen. Microbiol. 139:1147-1153.
13.	Hynes, R. K., and R. Knowles. 1983. Inhibition of chemoautotrophic nitrification by sodium chlorate and sodium chlorite: a reexamination. Appl. Environ. Microbiol. 45:1178-1182[Abstract/Free Full Text].
14.	Johnsen, R. I., O. Grahl-Nielsen, and B. T. Lunestad. 1993. Environmental distribution of organic waste from a marine fish farm. Aquaculture 118:229-244.
15.	Johnstone, B. H., and R. D. Jones. 1988. Effects of light and CO on the survival of a marine ammonia-oxidizing bacterium during energy source deprivation. Appl. Environ. Microbiol. 54:2890-2893[Abstract/Free Full Text].
16.	Jones, R. D., and M. A. Hood. 1980. Effects of temperature, pH, salinity, and inorganic nitrogen on the rate of ammonium oxidation by nitrifiers isolated from wetland environments. Microb. Ecol. 6:339-347.
17.	Jones, R. D., and R. Y. Morita. 1985. Survival of a marine ammonium-oxidiser under energy-source deprivation. Mar. Ecol. Prog. Ser. 26:175-179.
18.	Jorgensen, K. S., and N.-P. Revsbech. 1985. Diffusive boundary layers and the oxygen uptake of sediments and detritus. Limnol. Oceanogr. 30:111-122.
19.	Jukes, T. H., and C. R. Cantor. 1969. Evolution of protein molecules, p. 21-132. In H. N. Munro (ed.), Mammalian protein metabolism. Academic Press, New York, N.Y.
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Nitrogen Cycling and Community Structure of Proteobacterial -Subgroup Ammonia-Oxidizing Bacteria within Polluted Marine Fish Farm Sediments

Nitrogen Cycling and Community Structure of Proteobacterial $beta$ -Subgroup Ammonia-Oxidizing Bacteria within Polluted Marine Fish Farm Sediments