Microbial Diversity of the Brine-Seawater Interface of the Kebrit Deep, Red Sea, Studied via 16S rRNA Gene Sequences and Cultivation Methods

doi:10.1128/AEM.67.7.3077-3085.2001

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Applied and Environmental Microbiology, July 2001, p. 3077-3085, Vol. 67, No. 7
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.7.3077-3085.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Microbial Diversity of the Brine-Seawater Interface of the Kebrit Deep, Red Sea, Studied via 16S rRNA Gene Sequences and Cultivation Methods

Wolfgang Eder,¹^,^* Linda L. Jahnke,² Mark Schmidt,³ and Robert Huber¹

Lehrstuhl für Mikrobiologie und Archaeenzentrum, Universität Regensburg, D-93053 Regensburg,¹ and Institut für Geowissenschaften, Universität Kiel, D-24098 Kiel,³ Germany, and Exobiology Branch, NASA Ames Research Center, Moffett Field, California 94035²

Received 12 February 2001/Accepted 17 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The brine-seawater interface of the Kebrit Deep, northern Red Sea, was investigated for the presence of microorganisms usingphylogenetic analysis combined with cultivation methods. Understrictly anaerobic culture conditions, novel halophiles were isolated.The new rod-shaped isolates belong to the halophilic genus Halanaerobiumand are the first representatives of the genus obtained from deep-sea,anaerobic brine pools. Within the genus Halanaerobium, they representnew species which grow chemoorganotrophically at NaCl concentrationsranging from 5 to 34%. The cellular fatty acid compositions areconsistent with those of other Halanaerobium representatives,showing unusually large amounts of $Delta$ 7 and $Delta$ 11 16:1 fatty acids.Phylogenetic analysis of the brine-seawater interface sample revealedthe presence of various bacterial 16S rRNA gene sequences dominatedby cultivated members of the bacterial domain, with the majorityaffiliated with the genus Halanaerobium. The new Halanaerobium16S rRNA clone sequences showed the highest similarity (99.9%)to the sequence of isolate KT-8-13 from the Kebrit Deep brine.In this initial survey, our polyphasic approach demonstrates thatnovel halophiles thrive in the anaerobic, deep-sea brine poolof the Kebrit Deep, Red Sea. They may contribute significantlyto the anaerobic degradation of organic matter enriched at thebrine-seawaterinterface.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Hypersaline ecosystems are one of the most unusual and extreme environments on earth (15, 25, 36). Anaerobic, deep-seabrine pools, which are located along various tectonic rift systems,represent a special type of hypersaline environment. During thelast 50 years about 25 deep-sea brine pools (Fig. 1) with highlysaline waters were identified in the Red Sea, an ocean in statunascendi within the East African Rift Valley system (1, 6,11, 13, 14, 18, 46, 53, 60, 65). The brines ofthe Red Sea are typical athalassohaline waters which are in themain a reflection of the geology, geography, and topography ofthe areas where they develop (18, 25, 27). The high salinityis formed when seawater circulates through subbottom Miocene evaporitedeposits, obtaining geothermal heat and dissolved solids beforesurfacing in the depression of the deeps (1, 12, 62, 72).Characteristic of the brine pools is the formation of gradientsalong the brine-seawater interface, e.g., salinity, pH, temperature,and oxygen gradients. Brine pools of different origin are alsofound in the Gulf of Mexico (e.g., the Orca Basin) and in theMediterranean Sea (e.g., the Tyro, Bannock, or Urania Basin) (19,37, 44, 61, 63).

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FIG. 1. Outline of the Red Sea, showing representative brine pools. The topographical map was generated with the Online Map Creation program (Geomar, Kiel, Germany [http://www.aquarius.geomar.de]).

The Kebrit Deep (in Arabic, kebrit means sulfur) in the northern Red Sea was first explored during a Valdivia cruise in 1971and consists of a basin of approximately 1 by 2.5 km in size (27,52, 59). The deep is filled with a brine of 84 m in thicknessat a maximum depth of 1,549 m (27). At the brine-seawater interfaceof the Kebrit Deep there is a steep increase in salinity from4 to 26% (wt/vol) NaCl (within only 3 m), an increase in temperaturefrom 21.6 to 23.4°C (within about 7 m), an increase of the CH₄concentration from 50 nl/liter to 22 ml/liter, and a measurablebrine pool H₂S content of up to 12 to 14 mg of S/liter. Over thesame interface the pH drops from 8.1 to 5.5 and the O₂ concentrationdecreases from 3.2 ml of O₂/liter to zero (23, 27, 64).At the same time, the density gradient created at the brine-seawaterinterface acts as an in situ particle trap for organic and inorganicmaterials from the Red Sea water (27-29, 40, 57, 60, 66).

During the last 30 years, detailed geological and geochemical investigations were carried out in the Kebrit Deep. In contrast,information about the microbial communities of this deep is veryrare. Recently, novel bacterial and archaeal 16S rRNA gene sequenceshave been retrieved from brine sediments (21, 48, 50). Theseinvestigations showed that novel groups of Archaea and Bacteria(KB1 sequence group) thrive in the extreme environment of theKebrit Deep (21). The presence of archaeal methanogenesis isalso suggested by the biochemical characterization of C₄₀ isoprenoids,an archaeal biomarker, in sedimentary organic matter (45), andan apparent biotic methane oxidation at the brine-seawater interface(23). Biochemical investigations in similar brine pools (Orcaand Bannock Basins) indicated a high microbial potential at thebrine-seawater interface and suggest the presence of halophilicmicroorganisms within the brine (17, 22, 39, 40, 68).

A great diversity of microorganisms have been isolated from high-salinity environments, including aerobic and anaerobic organismsof the bacterial and archaeal domains (25). These halophilicBacteria include sulfate reducers (reference 4 and referencestherein) and anaerobic phototrophs, gram-positive heterotrophs,and cyanobacteria (references 8 and 25 and references therein).Some isolates, like Flexistipes sinusarabici, represent separatelineages (24). In addition, the Halanaerobiaceae, which representa monophyletic lineage within the Bacteria, are specifically adaptedto their high-salt milieu (49, 55, 71). The halophilic Archaeaknown to date comprise aerobic halophiles of the family Halobacteriaceaeand anaerobic methanogens of the family Methanosarcinaceae (16,26, 47).

The goal of this research was to assess, for the first time, the bacterial diversity of the brine-seawater interface of theKebrit Deep, Red Sea. In this initial survey, which is preliminary,a twofold approach was used. This includes (i) phylogenetic analysisof 16S rRNA gene sequences as indicators of prokaryotic diversityand (ii) isolation and cultivation of halophilic representativesto establish physiological and function potential within the ecosystemcommunity.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Sampling. Brine from the brine-seawater interface of the Kebrit Deep, Red Sea (Fig. 1), was sampled during RV Sonne cruise SO 121 in1997 using a rosette sampler equipped with 24 niskin bottles (10liters) and a conductivity-temperature-depths (CTD) unit for monitoringsalinity, temperature, transmission, and pressure (Sea-Bird Electronic,Bellevue, Wash.). The salinity of brine samples was measured witha hand refractometer (Atago, Tokyo, Japan). Microorganisms wereconcentrated by pumping anaerobic brine across a crossflow tangentialfiltration unit (Pellicon Kasettensystem; Millipore, Eschborn,Germany) (Fig. 2) under a CO₂ protective atmosphere (cell concentrationfactor, 400-fold). Concentrated brine sample KT-2 was reducedwith sodium dithionite (about 0.1 µM), and KT-3 was used withoutfurther treatment. In addition, sample KT-8 was taken from surfacesediment of the Kebrit Deep by a chain-sack dredge (station no.17034-2). The sample located near the brine-seawater interfaceconsisted of oily ore rocks and brine (salinity, 15.6%). The sampleswere transported to the laboratory by air at ambient temperatureand were stored at 4°C.

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FIG. 2. Schematic drawing of the anaerobic filtration system. The crossflow filtration unit was equipped with five Durapore membranes (pore size, 0.2 µm; filter surface, 0.46 m²) (Millipore). The cells were kept in suspension and were pumped under pressure over the filter surface. Before filtration, the complete system was flushed for 10 min with CO₂ to remove oxygen. During the filtration procedure, a protective atmosphere of CO₂ was maintained to prevent cellular damage due to oxygen sensitivity, to prevent precipitation of inorganic compounds, and to keep the pH of the sample constant. The concentrated brine was collected in tank 1; tank 2 was for storage. Brine flowed into the filtration unit at valve 1, concentrated cells exited at valve 2, and the filtrate outflow was at valve 4. Valve 3 is a closed valve.

Strains. Halanaerobium praevalens DSM 2228, Halothermothrix orenii DSM 9562, and Halanaerobacter lacunaris DSM 6640 were obtained fromthe Deutsche Sammlung von Mikroorganismen und Zellkulturen (DSMZ),Braunschweig, Germany, and were cultivated by using the indicatedDSMZmedia.

Culture conditions. Enrichment cultures from samples KT-2 and KT-3 (KT-2/3) and KT-8 were established in 28-ml serum tubes on board the RV Sonne.Brine used for enrichments was supplemented with various sterileorganic and inorganic compounds (e.g., yeast extract, peptone,NaNO₃, and Na₂SO₄) and chemically reduced by the addition of 1ml of 50% (vol/vol) H₂S per 10 ml of brine. In the laboratory,positive enrichments were transferred several times in supplementedbrine and then grown in a synthetic medium whose composition wasbased on a chemical analysis of a Red Sea brine-seawater interface(brine interface medium [BI medium]) (D. Garbe-Schönberg [Institutfür Geowissenschaften, Universität Kiel, Germany], personalcommunication). BI medium contained (per liter) 100 g of NaCl,5.11 g of MgSO₄ · 7H₂O, 2.0 g of CaCl₂ · 2H₂O, 107 mg of MgCl₂· 6H₂O, 19 mg of MnSO₄ · H₂O, 10 mg of SrCl₂ · 6H₂O, 2.7 mg ofFeCl₂ · 4H₂O, 0.075 mg of NaNO₃, 0.7 mg of ZnSO₄ · 7H₂O, 0.02mg of Na₂MoO₄ · 2H₂O, 100 mg of KH₂PO₄, and 1.0 g of NaHCO₃. ThepH was adjusted to 6.5 with HCl. The gas phase over the mediumin incubation tubes was replaced with N₂, and residual O₂ waschemically reduced by the addition of 1 ml of 50% (vol/vol) H₂Sper 10 ml of medium. Growth was determined by direct cell countingwith a Thoma chamber (depth, 0.02mm).

Cell masses of Halanaerobium praevalens, Halothermothrix orenii, Halanaerobacter lacunaris, and the novel isolates were obtainedby growth at 30°C (60°C for Halothermothrix orenii) with stirring(100 rpm) in an 80-liter enamel-protected fermentor (Bioengineering,Wald, Switzerland) pressurized with 300 kPa of N₂ (N₂-CO₂ [80:20,vol/vol] for Halanaerobacter lacunaris and Halothermothrix orenii).

Light and electron microscopy. Light microscopy, electron microscopy, and photography were carried out as described elsewhere (31).

Lipid analyses. Freeze-dried cells (about 1 g) were extracted twice using chloroform-methanol (2:1, vol/vol) under reflux for 1 h. Fatty acidmethyl esters (FAME) were prepared from a portion of the totallipid extract by a modification of the mild alkaline methanolysisprocedure of White et al. (67), which involves heating at 37°Cfor 1 h and extraction with hexane-chloroform (4:1, vol/vol).FAME were separated by thin-layer chromatography on Silica GelG plates (Merck, Darmstadt, Germany) using methylene chlorideas the solvent. Gas chromatographic analysis was done using aPerkin-Elmer model Sigma 3B equipped with a flame ionization detectorand a DB-5 megabore column (J&W Scientific, Folsom, Calif.), withmethyl tricosanoate as an internal standard. Double-bond positions,cis-trans configurations, and confirmations of cyclopropane ringswere determined with dimethyl disulfide adducts (69) using gaschromatography-mass spectrometry (35).

DNA extraction, PCR, and cloning. Nucleic acids were extracted from 120 ml of the brine-seawater interface sample KT-2 with the IsoQuick Nucleic Acid Extractionkit (ORCA Research, Bothell, Wash.) according to the manufacturer'sinstructions, followed by RNase treatment for 30 min and precipitationof the nucleic acids with 1 volume of isopropanol. The nucleicacids of the halophilic isolates were extracted as described elsewhere(7). PCR amplifications of the rRNA genes between Escherichiacoli positions (5) 9 and 1406 or 9 and 1512 (9bF, bacterialprimer; 1406uR and 1512uR, universal primers) were carried outas described previously (21). PCR products of sample KT-2 werepurified (Microcon 100; Amicon, Witten, Germany), and the 16SrRNA gene fragments were cloned into the pCR2.1 vector (Invitrogen,Leek, The Netherlands) according to the manufacturer's instructions.The resulting ligation products were used to transform E. coliTOP10F' cells. The presence of inserts of the appropriate sizein the transformants was identified by direct PCR screening; amplifiedribosomal DNA (rDNA) restriction analysis was performed as describedpreviously (21). Representative transformants were selectedbased on the fingerprinting pattern of the rRNA gene clones, andthe corresponding plasmid DNAs were obtained using a QIAprep SpinMiniprep kit (Qiagen, Hilden,Germany).

Sequencing of rRNA genes. 16S rRNA gene sequences of the halophilic isolates and 16S rDNA clone sequences of sample KT-2 were sequenced with an ABIPrism 310 capillary DNA sequencer (PE Applied Biosystems, FosterCity, Calif.), using the ABI Prism BigDye Terminator Cycle SequencingReady Reaction kit (Perkin-Elmer), at the Institute for Genetics,University of Regensburg, Regensburg, Germany. The bacterial sequenceswere determined using a set of specific and universal primers(21).

Phylogenetic analyses. For the analyses, an alignment of about 11,000 homologous full and partial primary sequences available in public databases(ARB project [41; W. Ludwig and O. Strunk, http://www.mikro.biologie.tu-muenchen.de/pub/ARB/documentation/arb.ps])was used. The new bacterial 16S rRNA gene sequences (1,365 to1,473 nucleotides) were fitted in the 16S rRNA tree by using theautomated tools of the ARB software package (http://www.mikro.biologie.tu-muenchen.de/pub/ARB/documentation/arb.ps).Distance matrix (Jukes-Cantor correction), maximum-parsimony,and maximum-likelihood (fastDNAml) methods were applied as implementedin the ARB software package (42, 51). Insignificant branchingpoints were shown by multifurication. Phylogenetic distances weredetermined using distance matrix analysis without applying a correctionfactor. Each sequence alignment was checked manually, and thesequences were analyzed with the CHECK_CHIMERA program of theRibosomal Database Project (43) to detect the presence of possiblechimericartifacts.

Nucleotide sequence accession numbers. The 16S rRNA gene sequences were submitted to EMBL and have been assigned accession numbers AJ309519 to AJ309527.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Transmission-temperature-depth profile of the brine-seawater interface. The data were collected during RV Sonne cruise SO 121. Figure 3 shows the transmission-versus-depth profile of the KebritDeep brine-seawater interface, including data for temperature.At a depth of 1,468 ± 3 m, 240 liters of brine was obtained (stationno. 17029-8; 24°43.16'N, 36°16.42'E). The original sample temperaturewas 22°C, with a pH of 6.5. O₂ was not detected, and the watersmelled strongly of H₂S. Over the 1-m length of the niskin bottlesthe salinity varied from 4.6% at the top to 9.6% at the bottom.Samples KT-2/3 were retrieved from the upper part of this brine-seawaterinterface, indicated by the beginning of an increase in temperatureand salinity (4.6 to 9.6%) and an decrease in transmission (Fig.3).

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FIG. 3. Transmission-temperature-depth profile of the brine-seawater interface of Kebrit Deep, Red Sea. The salinities at water depths of 1,465, 1,467, 1,469, 1,470, and 1,471 m (corrected depths) are 4.0, 4.2, 17.2, 24.5, and 26.0% (wt/vol) NaCl, respectively.

Enrichment and isolation. In order to isolate representative microorganisms from the Kebrit brine, enrichment cultures were established in 28-ml serumtubes on board ship by adding different sterile organic and inorganicnutrients directly to the brine. Two successful enrichments designatedKT-2/3-3 (from the brine-seawater interface, 1,468 ± 3 m) andKT-8-13 (from a brine surface sediment near the brine-seawaterinterface) were grown anaerobically in original brine supplementedwith 0.1% (wt/vol) thiosulfate and 0.01% (wt/vol) of a mixtureof equal parts of yeast extract, meat extract, peptone, and brainheart infusion (C-Org). In the laboratory, the enrichment cultureswere transferred several times in the original brine and theninto synthetic BI medium. From each enrichment culture, a singlecell, which was optically trapped by using a strongly focusedinfrared laser beam ("optical tweezers"), was separated undervisual control from the mixed culture and was grown as a pureculture (selected cell cultivation [2, 30, 32]). The purecultures KT-2/3-3 and KT-8-13 (for simplicity, designated theenrichment cultures) were chosen as representatives for the experimentsdescribed below. Unless indicated otherwise, the novel isolateswere cultivated in BI medium supplemented with 0.01% C-Org. Severalfurther enrichment cultures resulted in single clones after selectedcell cultivation, but they showed 16S rRNA gene sequences identicalto that of either KT-2/3-3 or KT-8-13 and therefore were not furthercharacterized (data notshown).

Morphology. Cells of isolates KT-2/3-3 and KT-8-13 were gram-negative, motile rods with rounded ends; the average cell length was 1 to2 µm, and the average cell width was 0.3 to 0.4 µm. Addition ofglucose (0.1%, wt/vol) resulted in an increase of the cell lengthup to 6.5 µm (for KT-8-13). During growth, cells of the two isolatesappeared singly or in pairs. No evidence of spore formation wasobserved. In transmission electron micrographs, the new isolatesexhibited monopolar, polytrichous flagellation with up to threeflagella per cell (Fig. 4).

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FIG. 4. Transmission electron micrographs of a dividing cell of Halanaerobium sp. strain KT-2/3-3 showing flagella (a) and of a single flagellated cell of Halanaerobium sp. strain KT-8-13 (b). The cells were air dried and platinum shadowed. Bars, 1 µm.

Growth and physiological characterization. Isolates KT-2/3-3 and KT-8-13 grew chemoorganoheterotrophically under strictly anaerobic culture conditions. Both isolateswere obligate halophiles, with an optimal NaCl requirement ofbetween 10 and 20% (wt/vol). They grew at NaCl concentrationsof between 5 and 34% at pH 6.5. In the presence of H₂ (5%, vol/vol),thiosulfate or S⁰ (but not sulfate) was reduced to H₂S without stimulating thegrowthrate.

Isolate KT-8-13 grew at temperatures of between 18 and 48°C, with an optimum of between 30 and 45°C. KT-8-13 was able to growheterotrophically on C-Org (0.001 and 0.1%) and brain heart infusion(0.01%). No growth was observed on glucose (0.1%), fructose (0.1%),saccharose (0.1%), maltose (0.1%), lactose (0.1%), xylose (0.1%),betaine (0.1%), cholesterol (0.1%), acetate (0.01%), yeast extract(0.01%), peptone (0.01%) (Merck), Trypticase-peptone (0.01%) (BBL),meat extract (0.01%), or Casamino Acids (0.01%). H₂S concentrationsof 0.5 to 50% (vol/vol) were tolerated by isolate KT-8-13.

Cellular fatty acid composition. The cellular fatty acid compositions of isolates KT-2/3-3 and KT-8-13 in comparison with those of representatives of threedifferent halophilic genera are given in Table 1. The novel bacterialhalophiles Halanaerobium praevalens, Halothermothrix orenii, andHalanaerobacter lacunaris were cultured under optimal growth conditions(see Materials and Methods) and were harvested in the exponentialgrowth phase. The FAME analysis of the Kebrit Halanaerobium isolates,KT-2/3-3 and KT-8-13, showed large amounts of 16:0 and 16:1 fattyacids and minor amounts of 18:0 and 18:1 fatty acids, consistentwith the data for Halanaerobium praevalens (Table 1) (71).The two Kebrit isolates contained a relatively large proportionof monounsaturated 16:1 with unusual bond positions at $Delta$ 7 and $Delta$ 11, closely matching the 16:1 isomer composition of Halanaerobiumpraevalens. Halothermothrix orenii contained little unsaturatedFAME, while Halanaerobacter lacunaris had 16:1 with the commonlyencountered $Delta$ 9 position but an unusual 18:1 for a bacterium, withthe bond at $Delta$ 9. Hopanoids were not detected in the organisms analyzed(data not shown).

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TABLE 1. Comparison of the cellular fatty acid compositions of isolates KT-2/3-3 and KT-8-13 with those of Halanaerobium praevalens, Halothermothrix orenii, and Halanaerobacter lacunaris

16S rRNA phylogeny. (i) Halophilic isolates. A comparative analysis of the 16S rRNA gene sequences revealed that isolates KT-2/3-3 and KT-8-13 belong to the Halanaerobiaceaewithin the monophyletic lineage of the Halanaerobiales (49,55). Further sequence alignments and phylogenetic analyses showedthe taxonomic and phylogenetic positions of the new isolates tobe among those of the members of the genus Halanaerobium (Fig.5). The sequence similarity of isolates KT-2/3-3 and KT-8-13 is97.1%. The sequence similarities of KT-2/3-3 and KT-8-13 to otherHalanaerobium species ranged from 95.7 to 99% and from 95.5 to99.4%, respectively.

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FIG. 5. 16S rRNA gene-based phylogenetic tree of the bacterial domain, including the 16S rDNA sequences from brine-seawater interface sample KT-2 and the 16S rRNA gene sequences of the new halophilic isolates from Kebrit Deep, Red Sea. The KB1 group marks a cluster of closely related environmental sequences, which were obtained from a sediment sample (depth, 1,515 m) of the Kebrit Deep (21). The topology of the tree is based on results of a maximum-parsimony analysis. Reference sequences were chosen to represent the broadest diversity of Bacteria. Only sequence positions that share 50% or more residues identical to the 16S rRNA sequences of a corresponding group were included for tree reconstruction. Accession numbers for the sequences are indicated. The scale bar represents 0.10 fixed mutation per nucleotide position.

(ii) Brine-seawater interface. Specific (9bF) and universal (1406uR) 16S rRNA primers were used to amplify bacterial sequences from bulk DNA derived fromthe brine-seawater interface sample KT-2 (salinity, 4.6 to 9.6%NaCl). About 40 clones were obtained from the extracted nucleicacids. After cloning, the 16S rRNA gene fragments were furthercharacterized by restriction endonuclease digestion. Based ona comparison of the restriction patterns on agarose gels, eightdifferent bacterial groups were identified. From a representativeof each restriction pattern group, the 16S rRNA gene sequencewas determined and aligned with 16S rRNA sequences derived fromthe ARB database. Clone sequences KT-2K20 and KT-2K29 (representing26% of the clones) were chimeras: KT-2K20 of KT-2K1 and KT-2K23/KT-2K28,and KT-2K29 of KT-2K1 and KT-2K38/KT-2K12.

The analysis of the clone sequences KT-2K1, KT-2K12, KT-2K23, KT-2K28, KT-2K34, and KT-2K38 showed a high phylogenetic diversitywithin the bacterial domain. The phylogenetic positions of thederived clone sequences were supported by the different tree reconstructionmethods (see Materials and Methods). KT-2K23 and KT-2K28 (together,41% of the derived clones) were affiliated with cultivated membersof the genus Halanaerobium (Fig. 5). They showed highest sequencesimilarity to Halanaerobium sp. strain KT-8-13 (99.9%), Halanaerobiumfermentans (99.3%), and Halanaerobium sp. strain KT-2/3-3 (97%).Sequence clones KT-2K1, KT-2K12, and KT-2K38 (representing 26%of the clones) showed the closest relationship to Clostridiumsubterminale or Propionibacterium acnes, whereas KT-2K34 (7% ofthe clones) is related to sequence clone PVB OTU 4 (U15116)within the $gamma$ -proteobacteria. The G+C contents of the rRNA genesequences range from 51 to 57%.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In brine-filled Red Sea deeps, the brine-seawater interface represents a unique microbial ecosystem mainly determined by asteep salt gradient (4 to 26% NaCl) within only a few meters.The combination of salt, oxygen, and pH gradients may be responsiblefor organisms specifically adapted to this environment. To date,nothing is known about the morphological and physiological featuresof these organisms. The presence of microorganisms in hypersalinebrines (e.g., the Gulf of Mexico and the Mediterranean Sea) wassuggested by biochemical investigations which included measurementsof ATP or CH₄, lipid analysis, and epifluorescence microscopy(17, 20, 40, 54, 68). The novel halophilic isolatesfrom the Kebrit Deep (KT-2/3-3 and KT-8-13) are the first organismsto have been cultivated and isolated from a brine-seawater interfaceor the deeper anaerobic, brinepool.

Based on 16S rRNA gene sequence comparisons, these Kebrit isolates were identified as members of the Halanaerobiales, a groupof anaerobic, halophilic, fermentative bacteria. The Halanaerobialesrepresent a separate lineage in the bacterial domain (49, 55).Within this order, the isolates KT-2/3-3 and KT-8-13 showed theclosest relationship to cultivated members of the genus Halanaerobiumand most likely comprise new species in the genus (3, 9,38, 49, 55, 56, 71). Prior to our investigations, membersof the genus Halanaerobium have been shown to occur only in sedimentsfrom salt lakes and offshore oil fields; this study thus increasesour knowledge of the ecological distribution of these organisms(3, 9, 55, 56). The results of the FAME analysis forthe new Halanaerobium species are consistent with the 16S rRNAdata in that the new species exhibit fatty acid patterns similarto those of Halanaerobium praevalens (71). The FAME are dominatedby 16:0 and 16:1 and minor amounts of 18:0 and 18:1. In contrastto Halothermothrix orenii, the new isolates show the presenceof large amounts of unsaturated fatty acids (Table 1) (10).The presence of relatively large amounts of $Delta$ 7 and $Delta$ 11 16:1 isvery unusual and may serve as a biomarker for Halanaerobium. Smallamounts of $Delta$ 11 16:1 are also present in type I methanotrophs;however, these bacteria also contain $Delta$ 8, $Delta$ 9, and $Delta$ 10 16:1 (33,34). Like most other Halanaerobium representatives, Halanaerobiumsp. strains KT-2/3-3 and KT-8-13 grew over a wide NaCl range (5to 34% NaCl). This physiological flexibility allows the organismsto grow within the salt gradient of the brine-seawater interfaceand in the highly saline lower brine pool. The brine-seawaterinterface also exhibits a density gradient which acts as an insitu particle trap for organic material (Fig. 3) (29, 40,57, 58, 66), providing an appropriate environmental nichefor heterotrophic bacteria. Indeed, these chemoorganotrophic halophilesmay contribute significantly to the anaerobic degradation of suspendedorganic material enriched at the brine-seawater interface of theKebrit Deep. However, the occurrence of Halanaerobium representativesis not restricted to the Kebrit Deep. Recently, a new member ofthe genus Halanaerobium (isolate S5L4, AJ309521) was obtainedfrom the brine-seawater interface (salinity, 24.2%) of the ShabanDeep, Red Sea (W. Eder and R. Huber, unpublishedresults).

For phylogenetic analysis, the brine sample was concentrated anaerobically on board ship using a crossflow tangential filtrationunit operated under a protective CO₂ atmosphere (Fig. 2). Twohundred forty liters of water of the brine-seawater interfacewas concentrated about 400-fold. Anaerobic sampling of the brineis essential to circumvent the precipitation of reduced inorganiccompounds such as Fe(II) in the presence of O₂ or the toxic effectof O₂ on strict anaerobes like methanogens (60, 70). Fromthe concentrated brine sample KT-2, the nucleic acids were extracted,and the 16S rRNA gene sequences were PCR amplified and cloned.The 16S rRNA gene fragments were further characterized by amplifiedrDNA restriction analysis, and different restriction pattern groupswere identified. The phylogenetic analysis of a representativeof each restriction group showed that the majority of the sequenceshad high sequence similarity to cultivated microorganisms withinthe bacterial domain. From the same bulk DNA, archaeal PCR productswere obtained, but these were not further investigated for thisstudy (Eder and Huber,unpublished).

Using different tree reconstruction methods (see Materials and Methods), the majority of the bacterial clone sequences representedby KT-2K23 and KT-2K28 showed the closest relationship with membersof the genus Halanaerobium (55) and exhibited the highest sequencesimilarity to the isolated Halanaerobium sp. strain KT-8-13. AlthoughKT-8-13 was enriched from the sedimentary portion of the brinepool, this sequence was not detected in a previous in situ analysisof the brine-sediment interface (21). That phylogenetic analysisidentified a deep-branching KB1 sequence group (Fig. 5) (21).This KB1 group could not be retrieved from the brine-seawaterinterface sample, suggesting that representatives of the KB1 groupare specifically adapted to the higher salinities within the lowerbrine body (Fig. 3) and the sediments (the salinity of the porewater is up to 26%), while KT-8-13, like KT-2/3-3, is more naturallyadapted to the interfaceenvironment.

	ACKNOWLEDGMENTS

We are grateful to Karl O. Stetter for stimulating and critical discussions. For helpful discussions we thank Reiner Botz,Roger Summons, and Gerald Maroske. Furthermore, we thank ReinhardRachel and Peter Hummel for electron microscopy and Thomas Hader,Konrad Eichinger, and Marcus Koch for technical assistance. Weare grateful for the valuable help of the crew on board the RVSonne (SO 121 cruise) and for the valuable support of cruise leaderPeterStoffers.

This work was financially supported by the BMBF (grant no. 03G0121B to Karl O. Stetter and grant no. 03G0121A to Peter Stoffers)and by the Fonds der Chemischen Industrie (to Karl O. Stetter).The work of L.L.J. was supported by a grant from NASA's Exobiologyprogram.

	FOOTNOTES

^* Corresponding author. Mailing address: Lehrstuhl für Mikrobiologie, Universität Regensburg, Universitätsstr. 31, D-93053Regensburg, Germany. Phone: 0941/943-3180. Fax: 0941/943-2403.E-mail: wolfgang.eder{at}biologie.uni-regensburg.de.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bäcker, H., and M. Schoell. 1972. New deeps with brines and metalliferous sediments in the Red Sea. Nat. Phys. Sci. 240:153-158.

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1.	Bäcker, H., and M. Schoell. 1972. New deeps with brines and metalliferous sediments in the Red Sea. Nat. Phys. Sci. 240:153-158.
2.	Beck, P., and R. Huber. 1997. Detection of cell viability in cultures of hyperthermophiles. FEMS Microbiol. Lett. 147:11-14[Medline].
3.	Bhupathiraju, V. K., M. J. McInerney, C. R. Woese, and R. S. Tanner. 1999. Haloanaerobium kushneri sp. nov., an obligately halophilic, anaerobic bacterium from an oil brine. Int. J. Syst. Bacteriol. 49:953-960[Abstract/Free Full Text].
4.	Brandt, K. K., B. K. C. Patel, and K. Ingvorsen. 1999. Desulfocella halophila gen. nov., sp. nov., a halophilic, fatty-acid-oxidizing, sulfate-reducing bacterium isolated from sediments of the Great Salt Lake. Int. J. Syst. Bacteriol. 49:193-200[Abstract/Free Full Text].
5.	Brosius, J., T. J. Dull, D. D. Sleeter, and H. F. Noller. 1981. Gene organization and primary structure of a ribosomal RNA operon from Escherichia coli. J. Mol. Biol. 148:107-127[CrossRef][Medline].
6.	Bruneau, L., N. G. Jerlov, and F. F. Koczy. 1953. Physical and chemical methods (+ Appendix), p. 99-112. Reports of the Swedish deep-sea expedition, vol. III. Physics and chemistry , no. 4.
7.	Burggraf, S., H. Huber, and K. O. Stetter. 1997. Reclassification of the crenarchaeal orders and families in accordance with 16S ribosomal RNA sequence data. Int. J. Syst. Bacteriol. 47:657-660[Abstract/Free Full Text].
8.	Caumette, P. 1993. Ecology and physiology of phototrophic bacteria and sulfate-reducing bacteria in marine salterns. Experientia 49:473-481[CrossRef].
9.	Cayol, J.-L., B. Ollivier, B. K. C. Patel, E. Ageron, P. A. D. Grimont, G. Prensier, and J. L. Garcia. 1995. Haloanaerobium lacusroseus sp. nov., an extremely halophilic fermentative bacterium from the sediments of a hypersaline lake. Int. J. Syst. Bacteriol. 45:790-797[Abstract/Free Full Text].
10.	Cayol, J.-L., B. Ollivier, B. K. C. Patel, G. Prensier, J. Guezennec, and J. L. Garcia. 1994. Isolation and characterization of Halothermothrix orenii gen. nov., sp. nov., a halophilic, thermophilic, fermentative, strictly anaerobic bacterium. Int. J. Syst. Bacteriol. 44:534-540[Abstract/Free Full Text].
11.	Charnock, H. 1964. Anomalous bottom water in the Red Sea. Nature 203:591[Medline].
12.	Craig, H. 1969. Geochemistry and origin of the Red Sea brines, p. 208-242. In E. T. Degens, and D. A. Ross (ed.), Hot brines and recent heavy metal deposits in the Red Sea. Springer-Verlag, New York, N.Y.
13.	Cruise report Menor 1. 1983. Preussag Meerestechnik, confidential report PREE-CR-03-4 (1403 AH). Ministry of Petroleum and Mineral Resources, Deputy Ministry for Mineral Resources, Jeddah, Saudi-Arabia.
14.	Cruise report Menor 2. 1984. Preussag Meerestechnik, confidential report PREE-CR-04-10 and PREE-CR-05-4 (1404AH und 1405AH). Ministry of Petroleum and Mineral Resources, Deputy Ministry for Mineral Resources, Jeddah, Saudi-Arabia.
15.	DasSarma, S., and P. Arora. 1999. Halophiles. In Embryonic encyclopedia of life sciences. [Online.] Nature Publishing Group, London, England. http://www.els.net.
16.	Davidova, I. A., H. J. M. Harmsen, A. J. M. Stams, S. S. Belyaev, and A. J. B. Zehnder. 1997. Taxonomic description of Methanococcoides euhalobius and its transfer to the Methanohalophilus genus. Antonie Leeuwenhoek 71:313-318.
17.	De Domenico, M., and E. De Domenico. 1989. Bannock Basin: first approach to water microbiology, p. 100-102. In M. B. Cita, A. Camerlenghi, and C. Corselli (ed.), Anoxic basins of the eastern Mediterranean: results of the third conference, Bergamo (Italy), December 14-16, 1988. Ricerca Scientifica Educazione Permanente, Mailand, Italy.
18.	Degens, E., and D. A. Ross. 1969. Hot brines and recent heavy metal deposits in the Red Sea. Springer-Verlag, New York, N.Y.
19.	de Lange, G. J., and H. L. ten Haven. 1983. Recent sapropel formation in the eastern Mediterranean. Nature 305:797-798.
20.	Dickins, H. D., and E. S. van Vleet. 1992. Archaebacterial activity in the Orca Basin determined by the isolation of characteristic isopranyl ether-linked lipids. Deep-Sea Res. 39:521-536.
21.	Eder, W., W. Ludwig, and R. Huber. 1999. Novel 16S rRNA gene sequences retrieved from highly saline brine sediments of Kebrit Deep, Red Sea. Arch. Microbiol. 172:213-218[CrossRef][Medline].
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