Distribution of Archaea in a Black Smoker Chimney Structure

doi:10.1128/AEM.67.8.3618-3629.2001

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Applied and Environmental Microbiology, August 2001, p. 3618-3629, Vol. 67, No. 8
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.8.3618-3629.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Distribution of Archaea in a Black Smoker Chimney Structure

Ken Takai,^* Tetsushi Komatsu, Fumio Inagaki, and Koki Horikoshi

Subground Animalcule Retrieval (SUGAR) Project, Frontier Research Program for Deep-Sea Extremophiles, Japan Marine Science and Technology Center, Yokosuka 237-0061, Japan

Received 26 February 2001/Accepted 30 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Archaeal community structures in microhabitats in a deep-sea hydrothermal vent chimney structure were evaluated through thecombined use of culture-independent molecular analyses and enrichmentculture methods. A black smoker chimney was obtained from thePACMANUS site in the Manus Basin near Papua New Guinea, and subsampleswere obtained from vertical and horizontal sections. The elementalcomposition of the chimney was analyzed in different subsamplesby scanning electron microscopy and energy-dispersive X-ray spectroscopy,indicating that zinc and sulfur were major components while anincreased amount of elemental oxygen in exterior materials representedthe presence of oxidized materials on the outer surface of thechimney. Terminal restriction fragment length polymorphism analysisrevealed that a shift in archaeal ribotype structure occurredin the chimney structure. Through sequencing of ribosomal DNA(rDNA) clones from archaeal rDNA clone libraries, it was demonstratedthat the archaeal communities in the chimney structure consistedfor the most part of hyperthermophilic members and extreme halophilesand that the distribution of such extremophiles in different microhabitatsof the chimney varied. The results of the culture-dependent analysissupported in part the view that changes in archaeal communitystructures in these microhabitats are associated with the geochemicaland physical dynamics in the black smokerchimney.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Since the discovery of deep-sea hydrothermal vents in 1979 (12, 15), various microorganisms have been isolated from globaldeep-sea hydrothermal vent environments (26, 27, 29). Hyperthermophilesand thermophiles, including members of both the bacterial andarchaeal domains, are the most frequently isolated microorganisms,and their physiological properties likely reflect the extraordinaryenvironmental settings of the deep-sea hydrothermal vents (9,10, 18, 23, 28, 42, 43, 53, 56, 60). In addition,recent culture-independent molecular approaches have revealedthe presence of as-yet-uncultivated thermophiles showing substantialphylogenetic diversity in the deep-sea hydrothermal vent environments(27, 38, 39, 44, 51). Relatively little is known aboutthe ecological significance and geomicrobiological function ofthe extremophilic microbial communities found, as the occurrence,abundance, and distribution of the microbial communities associatedwith the formation of diverse geochemical and physical gradientsremain to beelucidated.

A deep-sea hydrothermal vent chimney, formed by chemical interaction between cold seawater and hot vent water, is a distinctivestructure in the deep-sea hydrothermal fields and is largely composedof sulfide materials. In the chimney structures and the underlyingsulfide mounds, steep environmental gradients of temperature,pH, oxidation-redox potential, and various chemicals can be formedby equilibration between the vent water and the seawater, andthese provide diverse microhabitats for microbial communities.In addition, the presence of similar environmental gradients inthe subvent environment beneath the active hydrothermal seaflooris evident. Based on several microbiological, geochemical, andgeophysical observations, the possible existence of a subventbiosphere populated by hyperthermophilic microorganisms was predicted(14). Also, microbial ribosomal DNA (rDNA) showing substantialdiversity was recovered from black smoker vent water in the IhayaBasin, Okinawa Trough (51), at a temperature of >300°C, whichis far above the upper temperature limit for growth of even themost hyperthermophilic archaeon, Pyrolobus fumarii (113°C) (9).The microbial rDNA may serve as a genetic signature indicativeof the microorganisms thriving in the subvent habitats, conveyedthere by vent water. Hence, a hydrothermal vent chimney is anenvironment analogous to the subvent biosphere, and elucidationof its microbial community structure is likely to provide greatinsight into features of the subvent microbialecosystem.

The black smoker chimney structure investigated in the present study was obtained from a hydrothermal vent field located atthe PACMANUS site in the Manus Basin near Papua New Guinea ata depth of 1,644 m. This hydrothermal field was discovered in1991 (7), and a geological survey of the field and geochemicalcharacterization of the vent waters have both been performed (6,7, 16, 17). The results of the microbiological assessmenthave not yet been reported. Archaeal community structures in microhabitatspresent in the chimney structure were evaluated through the combineduse of culture-independent molecular analyses and enrichment culturemethods. The molecular techniques used in this study are PCR-basedterminal restriction fragment length polymorphism (T-RFLP) andrDNA clone analyses, and the data provided by these methods shouldbe carefully evaluated. However, the PCR-mediated molecular techniqueswill allow the possible detection and evaluation of a probablyvery low biomass of archaeal communities in the hardly accessibledeep-sea hydrothermal vent chimney. The distribution of archaealcommunities associated with the occurrence of discrete microhabitatsin the chimney structure and implications for the possible subventbiosphere arediscussed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Sample collection, subsampling, and chemical analysis. A chimney structure was obtained from a black smoker found in a hydrothermal field at the PACMANUS site in the Manus Basin(03°43.816'S, 151°40.016'E) at a depth of 1,644 m by means ofthe manned submersible Shinkai 2000 in a dive in 1999 (dive no.1151). The in situ temperature of the effluent black smoker ventwater was found to be over 250°C. The chimney structure was immediatelycooled and stored during 2 weeks in an anaerobic bag filled with100% N₂ at 4°C prior to subsampling in the laboratory. Duringthe storage, no apparent change was found in the appearance ofthe chimneystructure.

A description of the structure of the chimney and of the identification features of the subsamples is shown in Fig. 1. Subsamplingwas performed in an anaerobic chamber in an atmosphere of 10%H₂ and 90% N₂. Each of the subsamples was subjected to chemicalanalysis, nucleic acid extraction, microscopic observation, andcultivation of microorganisms. Subsamples I and II were obtainedfrom the top part of the chimney. A surface layer (thickness,1 to 2 mm) with white or gray weathering (subsample II) was moisturizedand grazed from the top part of the chimney, and the rest (subsampleI) was less moisturized and pulverized using a mortar and pestlewhich had been sterilized by heating in a dry oven (200°C). Asurface layer (thickness, 1 to 2 mm) with white, orange, or grayweathering (subsample III) was also obtained from the middle partof the chimney. The vent surface (subsample IV), which was black,solid, and crystalline and contained little water, was pulverizedusing a mortar and pestle. Subsamples V and VI were obtained fromthe inside structure of the root part of the chimney. The innerstructure (subsample V) was gray, soft, and porous and containeda considerable amount of water. The outer structure (subsampleVI) was black and solid and much less moisturized. The outer structurewas pulverized using a mortar and pestle.

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FIG. 1. Schematic drawings of the morphological and structural features of a black smoker chimney and the subsampling method used. (A) Appearance of the surface. (B) Vertical section of the whole chimney structure. (C) Horizontal section of the root part of the chimney. The part where each of the subsamples was taken and the preliminary morphological and structural features of the subsamples are indicated.

The elemental composition of the subsamples was analyzed by scanning electron microcopy and energy-dispersive X-ray spectroscopy(SEM-EDS). The grazed or pulverized samples were directly embeddedon specimen mounts using adhesive tape or electroconductives.After natural drying, the specimen was coated with osmium plasmato a thickness of 5 nm by using an osmium plasma coater. The coatedspecimen was observed using a JEOL JSV-5800LV scanning electronmicroscope at 15 kV and was analyzed using an energy-dispersiveX-ray spectrometer with an ultrathin window at 15 kV. NaCl, BaSO₄,BaO, BaS, ZnSO₄·7H₂O, ZnO, ZnS, and colloidal elemental sulfur(S⁰) (Nakarai Tesque, Kyoto, Japan) were used as referencesubstances.

Microscopic observation. A 2-g portion of the subsample was suspended in 6 ml of sterilized synthetic seawater (MJ) (46, 54) containing 3.7% (wt/vol)formaldehyde, and the mixture was vigorously agitated for 2 minusing a vortex mixer. The suspension solution was very brieflycentrifuged (3,000 × g), and the supernatant was filtered witha 0.22-µm-pore-size 13-mm-diameter polycarbonate filter (Advantec,Tokyo, Japan). The filter was stained by treatment with MJ seawatercontaining 4',6'diamidino-2-phenylindole (DAPI) (10 µg ml¹) or acridine orange (10 µg ml¹) at 4°C for 20 min. The filter was briefly rinsed in MJ seawaterand examined under epifluorescence using a Nikon Optishotmicroscope.

Extraction of nucleic acids. Microbial DNA was directly extracted from each subsample (approximately 5 g) using a Soil DNA Kit Mega Prep (MO BIO Laboratories,Inc., Solana Beach, Calif.), following the manufacturer's suggestedprotocol. Microbial RNA was extracted from a replicate aliquotof each of the samples used for DNA extraction. Approximately5 g of sample material was suspended in 3.5 ml of extraction buffer(pH 4.2) containing 25 mM sodium acetate, 5 mM EDTA, and 5% (wt/vol)sodium dodecyl sulfate. Then 2.5 g of sterile glass beads (0.1-mmdiameter; Sigma) and 3.5 ml of phenol equilibrated with extractionbuffer were added. The suspension was shaken on a bead beaterfor 2 min and incubated at 60°C for 1 h. The shaking treatmentwas repeated, and the suspension was centrifuged at room temperature.The lysate was extracted with phenol-chloroform-isoamyl alcohol(25:24:1, vol/vol/vol) and with chloroform-isoamyl alcohol (24:1,vol/vol). RNA was precipitated by adding 1.5 ml of 10 M ammoniumacetate and the same volume of isopropyl alcohol and was recoveredby centrifugation. The pellet was washed with 70% (vol/vol) ethanoland dissolved in filter-sterilized, distilled, deionized water.The total RNA was purified from the crude RNA solution using aRNeasy Midi Kit spin column (Qiagen, Valencia, Calif.). All plasticwareand all solutions used for RNA extraction and purification weretreated with 0.1% diethyl pyrocarbonate to inactivate nucleases.In order to check for laboratory contaminants, a blank tube (withno sample added) was processed as a negative control in the caseof both DNA and RNA extraction (57). RNA and DNA concentrationswere measured using aspectrophotometer.

Quantification of archaeal rRNA and the rDNA population. Quantification of archaeal rRNA in the whole microbial RNA assemblages extracted from the subsamples was performed by RNAdot blot hybridization. A dilution series of RNA samples (1, 0.5,and 0.25 ng µl¹) with 10 mM Tris-HCl (pH 7.5) were prepared, the RNA was denaturedat 100°C for 10 min, and the samples were cooled on ice. The denaturedRNA samples were dotted onto Hybond-N+ nylon membranes (AmershamPharmacia) and cross-linked to the membranes by exposure to 120mJ of UV light energy using a UV Stratalinker 1800 (Strategene,Torrey Pines, Calif.). The oligonucleotide probes (Uni1392R andArch915R conjugated at the 5' ends to digoxigenin) (52) andthe hybridization conditions used have been described previously(52). Quantification of the archaeal rDNA population in thewhole microbial DNA assemblages was performed by a quantitativefluorescent PCR method as previously described (52). An archaealrDNA mixture containing equal amounts of eight kinds of archaealrDNA (Haloarcula japonica, Palaeococcus ferrophilus, Pyrobaculumsp., Sulfurisphaera sp., pISA42, pISA48, pISA16, and pMC1A11)was used as a standard (52).

T-RFLP analysis of archaeal rDNA. In order to rapidly identify archaeal sequences in the subsamples, T-RFLP analysis of rDNA was performed (34). ArchaealrDNA was amplified by PCR using LA Taq polymerase (TaKaRa, Kyoto,Japan). The oligonucleotide primers used were Arch21F and Arch958R-FAM(13). Reaction mixtures were prepared in which the concentrationof each oligonucleotide primer was 0.1 µM and that of the DNAtemplate was 0.1 ng µl¹. Thermal cycling was performed using GeneAmp 9600 (Perkin-Elmer,Foster City, Calif.), and the conditions were as follows: denaturationat 96°C for 20 s, annealing at 50°C for 45 s, and extension at72°C for 120 s for a total of 30 cycles. In cases in which noapparent product was recovered after 30 cycles of reaction, thenumber of cycles was extended to 45 cycles. In the fewer cyclesof the reaction (20 and 25 cycles for 30 cycles and 35 and 40cycles for 45 cycles), no apparent product wasobtained.

Amplified rDNA from two separate reactions was pooled and subjected to agarose gel electrophoresis. The products were purifiedby means of a Gel Spin DNA purification kit (MO BIO). The DNAwas precipitated with ethanol and centrifuged, and the pelletwas resuspended in the distilled deionized water. The purifiedrDNA was digested with a restriction enzyme (HhaI). The terminalrestriction fragments (T-RFs) were analyzed using a model 377automated sequencer equipped with GeneScan software, version 3.0(PE Applied Biosystems, Foster City, Calif.). The precise lengthsof T-RFs were determined by comparison with an internal size standardadded to each digested sample. The electrophoresis conditionsand the procedures followed were those suggested in the manufacturer'sprotocol. The archaeal T-RFLP profiles from the subsamples wererepeatedly checked in a different series of experiments for PCRamplification, restriction enzyme reaction, andelectrophoresis.

Cloning and sequencing of archaeal rDNA. Archaeal rDNA was amplified by PCR using the same protocol as for T-RFLP analysis except for the use of a nonlabeled primerset of Arch21F and Arch958R. Amplified rDNA from two separatereactions was purified as described above. The purified rDNA wascloned in the vector pCR2.1 using the Original TA cloning kit(Invitrogen, Carlsbad, Calif.). The inserts were amplified bydirect PCR from a single colony using M13 primers (36), treatedwith exonuclease I and shrimp alkaline phosphatase (Amersham PharmaciaBiotech, Little Chalfont, Buckinghamshire, United Kingdom), anddirectly sequenced by the dideoxynucleotide chain-terminationmethod using a dRhodamine sequencing kit (PE Applied Biosystems)following the manufacturer's recommendations. The Arch21F primerwas used in partial sequencinganalysis.

Sequence and phylogenetic analyses. Single-strand sequences approximately 400 nucleotides in length were analyzed. The sequence similarity among all of the single-strandsequences was analyzed using the FASTA program equipped with DNASISsoftware (Hitachi Software, Tokyo, Japan). The rDNA sequenceshaving $>=$ 98% similarity as determined by the FASTA program wereassigned to the same clone type, and a representative sequenceof each clone type was applied to sequence similarity analysiswith databases by the gapped-BLAST method (1, 8). The databasesused for gapped-BLAST analysis were the prokaryotic small-subunit(SSU) rRNA database and the nonredundant nucleotide sequence databasesfrom GenBank, EMBL, andDDBJ.

Sequences of representative rDNA clones approximately 0.95 kb in length were determined from both strands. The data from therDNA clone libraries and the data from T-RFLP analysis were linkedby calculating the T-RF length for the sequenced clones. Cloneswith a T-RF length identical (within ±1 bp) to one found by T-RFLPanalysis were assigned to a T-RFLP ribotype. The sequences weremanually aligned to prokaryotic SSU rDNA data from the RibosomalData Project II (35) based on primary and secondary structureconsiderations and were also submitted to analysis using the ChimeraCheck program of the Ribosomal Data Project II to detect the presenceof chimeric artifacts. Phylogenetic analyses were restricted tonucleotide positions between the Arch21F and Arch958R primersthat were unambiguously alignable in all sequences. Neighbor-joininganalysis was performed using the PHYLIP package (version 3.5;obtained from J. Felsenstein, University of Washington, Seattle).Bootstrap analysis was used to provide confidence estimates forphylogenetic treetopologies.

Enrichment and MPN calculation. For enrichment cultures targeting members of the genus Thermococcus, MJYPS medium (56) was used and enrichment was performedat 55, 75, and 90°C. For enrichment cultures targeting halophilicmicroorganisms, including members of the genus Haloarcula, themedium (hemagglutinin [HA] medium) described by Ihara et al. (24)was used and enrichment was performed at 30 and 45°C. The three-tubemost-probable-number (MPN) method was employed to assess the populationsof viable cells obtained by enrichment from the subsamples. Themicroorganisms present in the most diluted of the series of culturesof MJYPS and HA media were isolated by the extinction-dilutionmethod. The partial sequences of the 16S rDNA were determinedand applied to sequence similarityanalysis.

Nucleotide sequence accession numbers. The sequences from this study are available through DDBJ under accession numbers AB052972 to AB052993.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Description of subsamples and chemical composition. Subsamples of the chimney structure were obtained from vertical and horizontal sections distinguished on the basis of morphologicalfeatures. In the case of hydrothermal vents with slowly flowingeffluent, it has often been observed that the top part of thechimney is covered with weakly packed materials, consisting ofchalcopyrite, pyrrhotite, and anhydrite on solid sulfide materials(21, 22, 33). The chimney investigated in the present studywas obtained from a black smoker with vigorously flowing effluent,and no such soft head-structure was observed. The vent surface,the interface with vent fluid, was formed by a solid, crystallinevent wall, which was observed throughout top to bottom of thechimney structure. The morphological features of the top partwere similar to those found on the vent surface. In the middleand root parts, four distinct inner structures were observed (Fig.1). Considering the features from inside towards the outer surface,a solid, crystalline vent wall, a grayish, porous soft structure,a black solid structure, and a thin orange layer approximately1 to 2 mm from the surface were recognized. The surface of thechimney was weathered and gray for the most part, with white ororange in some parts. These morphological features might be associatedwith geochemical and physical gradients of temperature, pH, oxidation-redoxpotential, and various chemicals formed in the chimneystructure.

The primary chemical composition of the subsamples was examined by SEM-EDS (Table 1). The whole chimney structure was foundto contain mainly elemental sulfur and zinc as the primary elements,suggesting that zinc sulfide is the main chemical fabric of thechimney. In the subsamples obtained from the surface of the chimney,a higher amount of elemental oxygen was observed. Although themolecular species containing oxygen was not identified, it seemedlikely that the higher proportion of oxygen detected in the elementalcomposition was consistent with the increasing amount of oxidizedmaterials on the outer surface of the chimney, indicating theoccurrence of relatively oxidative microhabitats in the exteriorzones of the chimney. In the weathered surface parts that werewhite and orange and in the orange subsurface layer, barium wasaccumulated at high levels while no significant change in theamount of calcium was observed.

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TABLE 1. Primary chemical composition of subsamples from a black smoker chimney obtained from the PACMANUS site^a

Microbial population density and nucleic acid extraction. The microbial population density was determined by direct counting of DAPI- and acridine orange-stained cells (Table 2).The highest population density was observed in the surface layerat the top part of the chimney (subsample II) and was 3.2 × 10⁷ cells g (wet weight)¹. The top part from which the surface was removed (subsample I)and the porous structure inside the chimney (subsample V) hadsomewhat higher population densities (1.0 × 10⁶ and 8.0 × 10⁵, respectively) than did the other subsamples (approximately 5× 10⁵).

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TABLE 2. Preliminary microbiological characterization of subsamples from a black smoker chimney at the PACMANUS site^a

Nucleic acids were directly extracted from the subsamples. Both DNA and RNA were isolated at concentrations in proportionto the observed population densities (Table 1). Based on theDNA yield from each sample and assuming an average cellular DNAcontent of 2 fg (2), the calculated microbial population densityin the subsamples was 8 × 10⁵ to 8.5 × 10⁷ cells g wet weight¹ and was thus in relatively good agreement with the populationdensities determined (Table 1).

Quantification of archaeal rRNA and rDNA populations. Archaeal rRNA and rDNA in the whole microbial RNA and DNA assemblages extracted from the subsamples were quantified by RNAdot blot hybridization and quantitative fluorogenic PCR (Table2). Throughout the subsamples, the proportion of bacterial rRNAor rDNA was higher than that of archaeal rRNA or rDNA in the wholemicrobial nucleic acid assemblages. However, the proportion ofarchaeal rRNA and rDNA varied among the subsamples. In the toppart of the chimney and the outer part of the inside structureof the root part, the proportion of both archaeal rRNA and rDNAwas increased while the proportion of the archaeal rRNA and rDNAin the other subsamples was a few percent or below the detectionlimit, in the whole microbial nucleic acid assemblages. Theseresults suggested that the sizes of the archaeal communities variedin different microhabitats in the black smokerchimney.

Molecular phylogenetic analyses. Profiles of archaeal ribotypes dominantly recovered from the DNA assemblages of the subsamples were examined by PCR-mediatedT-RFLP analysis (Fig. 2). Archaeal rDNA clones obtained from thesubsamples were characterized by partial sequencing (ca. 400 nucleotides)and sequence similarity analysis. The number of archaeal rDNAclones characterized varied from 44 to 65 for each of the samples(Table 3). In addition, sequences of representative rDNA clonesthat were approximately 0.95 kb in length were determined fromboth strands and were then applied to the phylogenetic analysis(Fig. 3). The data from the representative DNA clone sequencesand the data from T-RFLP analysis were linked by calculating theT-RF length for the sequenced clones.

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FIG. 2. Typical electropherograms of archaeal T-RFLP generated from rDNA with a labeled reverse primer and HhaI digest obtained from subsamples. The numbers on the peaks indicate major ribotypes commonly observed in various subsamples. Shown are a typical archaeal pattern from the top part of the chimney (subsample I) (A), the surface layer grazed from subsample I (subsample II) (B), the surface layer grazed from the middle part of the chimney (subsample III) (C), the vent surface (subsample IV) (D), the inner soft and porous structure in the root part of the chimney (subsample V) (E), and the outer black and solid structure in the root part of the chimney (subsample VI) (F).

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TABLE 3. Distribution of representative T-RFLP ribotypes and clone types of archaeal rDNA obtained from a black smoker chimney^a

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FIG. 3. Phylogenetic trees based on SSU rDNA sequences including various rDNA clones obtained from the black smoker chimney at the PACMANUS site in the Manus Basin. Each of the trees was inferred by neighbor-joining analysis of approximately 600 homologous positions of the rDNA sequence. (A) A tree indicating the phylogenetic relationship among the domains of Bacteria and Eucarya, the deep branches of uncultivated archaea, and the crenarchaeotic and euryarchaeotic kingdoms. (B) A tree indicating the phylogenetic organization among the hyperthermophilic crenarchaeota, Thermoproteales, Igniococcales, and Sulfolobales. (C) A tree indicating the phylogenetic relationship within the hyperthermophilic and thermophilic euryarchaeota and the possible thermophilic euryarchaeotic phylotypes. (D) A tree indicating the phylogenetic organization within the genus Haloarcula. The numbers on the branches represent the bootstrap confidence values. The scale bars indicate the expected changes per sequence position. Abbreviations indicate rDNA clones corresponding to uncultivated organisms derived from the following environments: pMC1A, pMC2A, pISA, and pIVWA from deep-sea hydrothermal vent environments (51); pOWA and pUWA from shallow marine hydrothermal vent water and terrestrial acidic hot spring water, respectively (55); pJP and pSL from sediments in Yellowstone National Park hot springs (3, 4); CRA and APA from deep-sea sediments (59); pHGPA from deep subsurface geothermal water (50); VC2.1 Arc from an in situ growth chamber (Vent Cap) deployed at a deep-sea hydrothermal vent (44); and pPACMA from a black smoker chimney at the PACMANUS site in the Manus Basin.

The molecular techniques used in this study were the PCR-based T-RFLP and rDNA clone analyses, and the data provided by thesemethods did not completely represent the archaeal community structuresthat occurred in the microhabitats of the chimney. In addition,unstable and strongly biased results have been pointed out inthe nonoptimized experiments using PCR-mediated T-RFLP and rDNAclone analyses (37, 41). The data obtained should be carefullyestimated.

In both T-RFLP and rDNA clone analyses, the structure of archaeal rDNA phylotypes was varied in the subsamples from differentmicrohabitats (Fig. 2 and Table 3). In the combined characterizationof T-RFLP and rDNA clone analyses, most of the major T-RFs foundin different subsamples had the corresponding archaeal phylotypesidentified by rDNA clone analysis, while no archaeal rDNA phylotypecoincident with T-RF designated as ribotype 1 or 2 was found throughoutall the subsamples (Fig. 2 and Table 3). In addition, there werecases in which the rDNA clones that corresponded to the T-RFsfound in the T-RFLP analysis were not obtained from the same subsamplein the rDNA clone analysis. This nonconformity between the T-RFLPprofiles and rDNA clone compositions might result from the unavoidablecloning bias in Escherichia coli or from the underestimation inthe limited number of rDNA clonessequenced.

The top part of the chimney (subsamples I and II) and the surface layer of the middle part (subsample III) contained a varietyof rDNA clones phylogenetically belonging to both Crenarchaeotaand Euryarchaeota (Table 3). An archaeal rDNA clone, pPACMA-Y,recovered from the archaeal rDNA clone libraries of the top partof the chimney, was phylogenetically associated with one of thedeepest branches within the domain of Archaea conventionally namedthe Marine Hydrothermal Vent Group (MHVG) (Fig. 3A). The T-RFprobably representing the deeply branched archaeal phylotype wasdetected in the top part of the chimney (subsamples I and II),the surface layer of the middle part (subsample III), and thevent surface (subsample IV) (Fig. 2). The archaeal phylotypespredominantly obtained from the top part of the chimney were affiliatedwith the clusters of Igniococcales, Thermococcales, and the uncultivatedDeep-Sea Hydrothermal Vent Euryarchaeotic Group (DHVEG) (Fig.3B and C). The archaeal rDNA clones affiliated with Igniococcaleswere especially closely related to the most hyperthermophilicarchaeal isolates, such as Pyrolobus (9), Pyrodictium (42),and Hyperthermus (60), capable of growth at or above 110°C (Fig.3B). All of the Thermococcales rDNA clones obtained from the chimneywere closely related with Thermococcus, and no Pyrococcus-typeclones were detected (Fig. 3C). The archaeal rDNA clones, pPACMA-M,-Q, -W, -P and -V, were clustered into a certain phylogeneticgroup consisting of only uncultivated environmental clones obtainedfrom geologically and geographically distinct deep-sea hydrothermalvent environments (44, 51) (Fig. 3C). The proportion of Igniococcalesphylotypes was reduced in the rDNA clone libraries from the surfacelayer samples (subsamples II and III), while the proportion ofrDNA clones phylogenetically associated with Thermococcus andDHVEG was greater in the surface zone (Table 3). These proportionchanges found in the rDNA clone analysis were also indicated bythe changes of T-RF signals (ribotypes 5, 6, 7, and 10) representingthe archaeal phylotypes (Igniococcales, Thermococcus, and DHVEG)in the T-RFLP analysis (Fig. 2).

In the vent surface (subsample IV), most of the archaeal rDNA phylotypes provided by rDNA clone analysis were Igniococcalesmembers (Table 3 and Fig. 3B). The dominant occurrence of thesephylotypes was clearly represented by a large single peak of ribotype5 in the T-RFLP analysis (Fig. 2). In addition, the presence ofribotype 4 was detected in the vent surface (Fig. 2), which matchedwell with the recovery of rDNA clones phylogenetically relatedwith Halobacteriales (Table 3).

In the inside structures of the chimney (subsamples V and VI), the major archaeal phylotypes found in the rDNA clone analysisshifted from hyperthermophilic groups of phylotypes to an extremelyhalophilic group of phylotypes within Halobacteriales (Table 3).These shifts in the archaeal rDNA clone community structure wereconsistent with the shifts in the ribotype structure revealedby the results of T-RFLP analysis (depletion of signatures ofribotypes 5 and 6 corresponding to rDNA clones of Igniococcalesand Thermococcales, respectively, and predominance of ribotypes3 and 4 representing Halobacteriales rDNA clones) (Fig. 2). Inthe phylogenetic analysis, all of the archaeal rDNA clones relatedwith Halobacteriales were located within the phylogenetic clusterof the genus Haloarcula (Fig. 3D). The phylogenetic placementof the Haloarcula rDNA clones obtained from the inside structuresof the chimney was divided mainly into two lineages. This dispersionand the relatively high divergence of the Haloarcula rDNA clonesequences could be due to the heterogeneity of the rRNA genesobserved in Haloarcula species (40). The archaeal rDNA clonepPACMA-N distantly related to any other archaeal rDNA sequencesknown so far (Fig. 3C) was detected at a small proportion in variousmicrohabitats both in the rDNA clone analysis and the T-RFLP analysis(Table 3 and Fig. 2). The results obtained from the molecularphylogenetic analyses indicated that different archaeal phylotypestructures consisting mainly of hyperthermophilic and extremelyhalophilic phylotypes were distributed in different microhabitatsin the black smokerchimney.

Enrichment and MPN calculations. In order to support the apparent distribution of different archaeal community structures indicated by culture-independentmolecular phylogenetic analyses, enrichment cultures of viablehyperthermophilic and halophilic microbial populations were preparedand MPN calculations were performed. Techniques for cultivationof Thermococcus and Haloarcula members, among the archaeal phylotypesidentified through molecular analyses, are relatively well established(5, 11, 45). Table 4 shows the viable-cell counts of Thermococcusmembers and halophilic microorganisms cultivated at several temperaturesin MJYPS and HA media. The microorganisms that grew in the mostdiluted series of cultures in MJYPS medium at 50 or 75°C containingsubsample II or in HA medium at 30°C containing subsample V wereisolated by the extinction-dilution method. Based on the resultsof similarity analysis of partial rDNA sequences, the microorganismsthat grew in MJYPS medium at 50 and 75°C were found to be Thermococcusspecies (Thermococcus spp. PACM50 and PACM75, shown in Fig. 3C).However, the microorganism that grew in HA medium at 30°C wasidentified as a Halomonas sp. (its partial 16S rDNA sequence had98.5% similarity with that of Halomonas meridiana [25]), a memberof the Bacteria, not the Archaea. HA medium contains approximately16% (wt/vol) NaCl or 20% total salts, which is within the rangefor growth of not only Haloarcula spp. but also of Halomonas spp.(58). In addition, no archaeal rDNA was detected by PCR analysisof DNA extracts from any of the enrichment cultures in HA mediumat any cultivation temperature. These results indicated that theviable cell counts obtained by the MPN method in the case of culturesusing HA medium represented the halophilic bacterial population,not the Haloarcula population. Although no viable cells of thegenus Haloarcula were recovered from any of the subsamples, thefindings obtained from the enrichment cultures supported the viewthat a viable Thermococcus population was present in the surfacelayers and that preferential colonization of the inside structuresof the chimney by halophilic microorganisms occurred.

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TABLE 4. Viable-cell counts of Thermococcus members and halophilic microorganisms calculated by three-tube MPN cultivation method^a

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The distribution of archaea in a black smoker chimney structure was analyzed by culture-independent, molecular phylogenetictechniques. The combined use of rRNA dot slot hybridization, quantitativefluorogenic PCR, T-RFLP, and rDNA clone analysis revealed thatthe archaeal phylotype community was significantly altered interms of size and structure with microhabitats varying at severalcentimeters distance in the deep-sea hydrothermal vent chimney.The occurrence of discrete archaeal phylotype communities waslikely associated with the formation of environmental gradientsof temperature, pH, oxidation-redox potential, and various chemicalsin the chimney structure, even though the measurement of the gradientswas not completely determined in thisstudy.

The occurrence of discrete microbial communities in deep-sea hydrothermal vent environments was first reported by Harmsenet al. (19) after applying enrichment culture and whole-cellfluorescence in situ hybridization (FISH) techniques (20) toanalysis of black smoker chimneys obtained from the Mid-AtlanticRidge. It was demonstrated that the microbial community densitywas varied in subsamples obtained from different parts of a chimneystructure and that the top part had the highest density (19).In addition, the increased density of the total archaeal populationin the top part of the chimney was observed by using the fluorescencein situ hybridization technique, and the preferred colonizationpatterns of potential Thermococcales members in the surface areaand of potential Igniococcales members in the top parts and thevent area were indicated by enrichment culture techniques (19).A similar distribution pattern of microbial communities was observedin our analysis of archaeal community structures in differentmicrohabitats of a black smoker chimney from the Manus Basin,which is geologically and geographically distinct from those inthe Mid-Atlantic Ridge. These features of the distribution ofmicroorganisms commonly observed in different deep-sea hydrothermalvent systems provide an important general aspect to be consideredin assessment of the global deep-sea hydrothermal vent microbialecosystem.

Significant changes in microbial abundance, diversity, and community structure associated with environmental gradients inhydrothermal environments have also been observed in a seriesof investigations focusing on a shallow marine hydrothermal ventsite as a model system (47-49). Through the use of molecular techniques,an increased abundance of the archaea was found in the activeventing area and complex, active, bacterial communities becamepredominant with increasing distance from the venting point (47-49).At the shallow marine hydrothermal vent site, temperature andpH ranging from approximately 70°C at pH 5 to 20°C at pH 7 wereformed over a distance of several meters (47). The potentialimpact of the environment on a microbial community might be muchmore intense in deep-sea hydrothermal systems, since gradientsare expected to exist in the range of approximately 300°C at pH3 to 4°C at pH 6 to 7 in the case of a black smoker investigated(16, 17) and from 350 to 400°C to 4°C in the case of the typicalmidocean-ridge systems (21). In the range of such extraordinarythermal gradients of the deep-sea vents, the archaeal componentsmay play a much more important role in the formation and activityof a microbial community than in the shallowvents.

The existence of a diversity of archaea in the deep-sea hydrothermal vent environments has been demonstrated through a numberof enrichment and isolation attempts to date (9, 10, 18,23, 28, 42, 43, 53, 56, 60). Additionally, culture-independent,molecular approaches have revealed that a greater diversity ofarchaea are predominantly present and remain unidentified in termsof their physiological properties and metabolic functions (44,51). This study is the first report in which the distributionof discrete archaeal communites in different microhabitats ofa black smoker chimney was demonstrated by using culture-independent,molecular phylogenetic analysis. In this study, it was revealedthat members of Thermococcus and members of the DHVEG are abundanton the chimney surface. The coexistence with the hyperthermophilesThermococcus, the wide distribution in the various deep-sea hydrothermalvents, the relatively short branch length in the phylogenetictree (Fig. 3C), and relatively high G+C content of the rDNA (57.6to 60.2%) of the uncultivated DHVEG may represent the thermophilyin this group of uncultivated archaea. Likewise, the deeply branchedphylotype pPACMA-Y, phylogenetically related to the MHVG, mightat least represent thermophily as its distinctive physiologicalfeature, as described previously (51).

The discovery of a sizable population of extremely halophilic archaea in the inside structures of the chimney was the moststriking finding in this work. Kaye and Baross have reported findinghalotolerant bacteria belonging to the genera Halomonas and Marinobacterat high incidence in a variety of samples obtained from deep-seahydrothermal vent environments (30). We also obtained here aculturable population of Halomonas from the inside structuresof the chimney. The halophilic bacteria are abundant in deep oceanwater and may be contaminated from the ambient seawater aroundthe deep-sea hydrothermal vent (30). Given that the halophilicbacterial population, including Halomonas sp. cultured from theinside structure of the chimney, is derived from the ambient seawater,there might be obtained a similar or higher abundance of culturesfor Halomonas spp. from the surface of the chimney exposure tothe seawater. The discovery of extremely halophilic archaeal rDNAand successful cultivation of halophilic microorganisms were achievedspecifically from the inside structures of the chimney. It seemslikelier, therefore, that the halophilic bacterial cultures andthe genetic signatures for extremely halophilic archaea are derivedfrom microbial communities dwelling in the microhabitats thatoccurred in the inside structures rather than from contaminatedmicrobial communities. Since no positive cultivation of the extremelyhalophilic archaea represented by rDNA phylotypes from the insidestructures was achieved, the viability of the extremely halophilicarchaeal population remained uncertain. However, the discoveryof extremely halophilic archaeal rDNA and the successful cultivationof halophilic bacteria suggest that partially hypersaline microhabitatsallowing the survival or growth of halophilic archaea and bacteriaoccur in the chimney structure. Furthermore, the recovery of hyperthermophilicand extremely halophilic archaeal rDNA phylotypes from the interfacewith the vent fluid and the interior structures of the chimneyleads to the hypothesis that the microbial communities in themicrohabitats of the chimney are provided from the microbial populationthriving beneath the active hydrothermal floor, the subventbiosphere.

Based on several microbiological, geochemical, and geophysical observations, Deming and Baross proposed the possible existenceof a hyperthermophilic subvent biosphere beneath the active hydrothermalvent fields (14). The relatively high density of microbial cellsand the detection of microbial rDNA in the black smoker vent waterat a temperature of >300°C also support the occurrence of a sizablemicrobial population in the subvent environment of the hydrothermalsystem in Ihaya Basin, Okinawa Trough (51). Since the deep oceanwater infiltrating this system consistently replenishes foreignmicroorganisms and nutrients in the environments, it is difficultto identify the exclusively indigenous microbial components andactivities in the subvent biosphere. However, extreme halophilesas well as hyperthermophiles are the possible indigenous microorganismsin the subvent biosphere. The physiological and metabolic diversityof known hyperthermophiles allows them to become accustomed toa variety of microhabitats in the subvent, most of which are extraordinaryhigh-temperature environments, as in the case of the chimney structure.In addition, the formation of brines or salt deposits in deep-seahydrothermal systems has been proposed (30-32). These brines orsalt deposits provide suitable microhabitats for the extremelyhalophilic archaea. The global distribution of extremely halophilicarchaea as well as of hyperthermophilic Thermococcales membershas been observed in nonhydrothermal pelagic subseafloor sedimentsand the subseafloor methane hydrate core samples (our unpublishedresults). The distribution of archaeal components found in thedeep-sea hydrothermal or the subvent environments in global subseafloormicrobial communities may shed light on the origin of the subsurfacemicroorganisms and the biogeographical propagation of hyperthermophilesand extreme halophiles. These are the foci of our futureefforts.

	ACKNOWLEDGMENTS

We thank the captain and crew of the R/V Natsushima and the DSV Shinkai 2000 operations group for their technical expertise.We also thank Katsuyuki Uematsu for assistance in analysis ofSEM-EDS and Wayne R. Bellamy for editing English usage in themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Deep-Sea Microorganisms Research Group (DEEP-STAR), Japan Marine Science and TechnologyCenter (JAMSTEC), 2-15 Natsushima-cho, Yokosuka 237-0061, Japan.Phone: 81-468-67-3894. Fax: 81-468-66-6364. E-mail: kent{at}jamstec.go.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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