Genetic Diversity of the Biofilm Covering Montacuta ferruginosa (Mollusca, Bivalvia) as Evaluated by Denaturing Gradient Gel Electrophoresis Analysis and Cloning of PCR-Amplified Gene Fragments Coding for 16S rRNA

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Applied and Environmental Microbiology, September 1998, p. 3464-3472, Vol. 64, No. 9
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Genetic Diversity of the Biofilm Covering Montacuta ferruginosa (Mollusca, Bivalvia) as Evaluated by Denaturing Gradient Gel Electrophoresis Analysis and Cloning of PCR-Amplified Gene Fragments Coding for 16S rRNA

David C. Gillan,¹^,^* Arjen G. C. L. Speksnijder,² Gabriel Zwart,² and Chantal De Ridder¹

Laboratoire de Biologie Marine, Université Libre de Bruxelles, Brussels, Belgium,¹ and Centre for Limnology, Netherlands Institute of Ecology, Nieuwersluis, The Netherlands²

Received 5 January 1998/Accepted 12 May 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The shell of the bivalve Montacuta ferruginosa, a symbiont living in the burrow of an echinoid, is covered with a rust-coloredbiofilm. This biofilm includes different morphotypes of bacteriathat are encrusted with a mineral rich in ferric ion and phosphate.The aim of this research was to determine the genetic diversityand phylogenetic affiliation of the biofilm bacteria. Also, thepossible roles of the microorganisms in the processes of mineraldeposition within the biofilm, as well as their impact on thebiology of the bivalve, were assessed by phenotypic inference.The genetic diversity was determined by denaturing gradient gelelectrophoresis (DGGE) analysis of short (193-bp) 16S ribosomalDNA PCR products obtained with primers specific for the domainBacteria. This analysis revealed a diverse consortium; 11 to 25sequence types were detected depending on the method of DNA extractionused. Individual biofilms analyzed by using the same DNA extractionprotocol did not produce identical DGGE profiles. However, differentbiofilms shared common bands, suggesting that similar bacteriacan be found in different biofilms. The phylogenetic affiliationsof the sequence types were determined by cloning and sequencingthe 16S rRNA genes. Close relatives of the genera Pseudoalteromonas,Colwellia, and Oceanospirillum (members of the $gamma$ -Proteobacterialineage), as well as Flexibacter maritimus (a member of the Cytophaga-Flavobacter-Bacteroideslineage), were found in the biofilms. We inferred from the resultsthat some of the biofilm bacteria could play a role in the mineralformation processes.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Bacteria are widespread in the sea and can colonize virtually any submerged substrate, whatever its nature (inert or living)(3, 5). In this context, a biofilm may develop and forma microbial community in which several types of microorganismscoexist and interact (5). Body surfaces of marine organismsare often colonized by bacteria which are termed epibionts andare considered symbionts sensu Kinne (this general term includesparasitism, commensalism, mutualism, and phoresis) (38). Theepibiotic coating can be complex when several types of microorganismsshare the same surface (33); moreover, the composition of thecommunity may change with time. Observations of epibiotic microbialcommunities have raised questions about biotic interactions betweenthe microorganisms and the living substrate (i.e., the host organism)and between the microorganisms themselves. Understanding theseinteractions is an important step in explaining the functioningof a microbial community on a particular substrate. Basically,to do this, the coexisting microorganisms must be identified andtheir metabolic abilities must be determined.

In studies of bacterial symbiosis and of microbial communities in general, microbiologists have long been constrained by theuse of traditional methods (cultivation and/or microscopy). Thesetraditional methods are essential for understanding the biologyof microbial communities, but it is known that they have limitedusefulness for revealing in situ microbial diversity (47). Consequently,the occurrence of epibiotic bacteria on marine organisms and thecomposition, structure, specificity, and stability of the epibioticbacterial communities known today remain for the most part unexplored.Genetic characterization of microbial diversity through amplificationand sequence analysis of the 16S rRNA genes (rDNAs) has been successfulin a wide range of environments (4, 8, 9, 21, 29,40, 44, 71). To date, only a few molecular studies of marineepibiotic microbial communities have been performed; some of thehosts that have been studied are the nematode Laxus sp. (55),the hydrothermal vent polychaete Alvinella pompejana (33), theshrimp Rimicaris exoculata (54), the gutless oligochaete Inanidrilusleukodermatus (13), and the seagrass Halophila stipulacea (73).

Montacuta ferruginosa is a small marine bivalve (length, ca. 7 mm) that lives in the burrow of the echinoid Echinocardiumcordatum (22). Each burrow generally contains one to seven bivalves,but up to 18 bivalves may share the same burrow (42). A typicalrust-colored coating covers the shell of M. ferruginosa and thespecific epithet refers to this coating. The coating is a partiallymineralized biofilm (ferric minerals rich in phosphate) made upof three superimposed layers: (i) a superficial layer that isessentially microbial and partially iron encrusted, (ii) a middlelayer with microorganisms that are deeply iron encrusted, and(iii) a deep layer that is essentially mineral and apparentlylacks microorganisms (27, 28). Although the predominant morphotypesof the biofilm are filamentous bacteria that resemble membersof the Beggiatoales (28), none of the bacteria has been identifiedor cultured.

The aim of the present work was to study the phylogenetic diversity of the M. ferruginosa biofilm bacteria. To obtain a globalview of the bacterial diversity of the biofilm, we used the denaturinggradient gel electrophoresis (DGGE) approach (48), and to obtainphylogenetic information, we used the classic cloning-sequencingapproach. We restricted our analyses to the domain Bacteria (51)by using specific primers. On the basis of the phylogenetic informationobtained, the major metabolic abilities of the epibiotic bacteriawere tentatively inferred in order to understand the potentialrole of these organisms in iron precipitation and their impacton the biology of the bivalve.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Samples. Specimens of M. ferruginosa (Montagu, 1803) were collected intertidally from the burrows of E. cordatum (Pennant, 1777) (Echinoidea,Spatangoida) at Wimereux (Pas-de-Calais, France) during Septemberand October 1996. The bivalves that shared the same burrow werenoted. In the laboratory, the bivalves were briefly rinsed insterile seawater (filter sterilized with 0.22-µm-pore-size filters)and measured (anteroposterior axis). The presence of filamentousbacteria (Beggiatoales-like bacteria) was determined for eachbivalve with a binocular microscope, and the levels of these bacteriawere estimated as follows: 0, no filaments; $-$ , few filaments;and +, abundant filaments. The biofilms were then scraped offeach shell with a sterile blade. Then, two sets of samples wereprepared; in one set the biofilms were pooled (pooled biofilmsamples), and in the other set they were kept individually (individualbiofilm samples). Two samples of pooled biofilms (samples E1 andE2) were prepared from a mixture of 60 biofilms; the mixture wasdivided into two parts that were suspended in 500 µl of TE buffer(10 mM Tris, 1 mM EDTA; pH 8.0). The two samples of pooled biofilms(samples E1 and E2) were subjected to different genomic DNA extractionprotocols. The individual biofilm samples were separately suspendedin 15 µl of TE buffer. Twenty individual samples were prepared.All 22 samples were then stored at $-$ 80°C.

DNA extraction. Different DNA extraction protocols, including both chemical disruption and physical disruption of bacterial cells, were testedpreviously (unpublished data). Only physical methods were usedin this study because they successfully extracted DNA from verysmall quantities of material. The following two physical methodswere used to extract DNA from the pooled biofilm samples: freeze-thawingfor sample E1 and bead beating for sample E2. Genomic DNA of themajor biofilm bacteria should have been obtained with these twomethods (the bacteria were efficiently lysed by the treatments,particularly by the bead-beating treatment). As the freeze-thawingmethod was very simple and very efficient (it resulted in morebands during DGGE than the other method), it was used to extractDNA from the individual biofilm samples. The freeze-thawing methodincluded four freeze-thaw cycles ( $-$ 196 and 80°C). The bead-beatingmethod included one cycle of bead beating with a Mini Beadbeater(Biospec Products). Bead beating was performed for 30 s at 5,000rpm after 0.5 g of zirconium beads (diameter, 0.1 mm) was added.Lysis of cells was checked by microscopy. After the lysis treatments,1- or 5-µl portions of the uncentrifuged mixtures were used directlyas template DNA for the PCR.

PCR amplification. The extracted DNA of the two pooled biofilm samples were used in two different PCR (62). For cloning, the nearly complete16S rDNA was amplified with primers 27F and 1492R, which are specificfor the domain Bacteria. For DGGE analysis, a 193-bp rDNA fragmentwas amplified with primers GM5F-GC-clamp and 518R. The 193-bpfragment spans the V3 region of the 16S rRNA (49). The GC clampwas a 40-nucleotide GC-rich sequence added so that the meltingbehavior of the DNA fragments during the DGGE analysis would bestable (48). The sequences of the primers are shown in Table1.

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TABLE 1. Primers used in this study

The PCR amplification procedure used for cloning was performed with an OmniGene temperature cycler as follows. Each mixturecontaining 5 µl of template DNA, each primer at a concentrationof 0.5 µM, each deoxynucleoside triphosphate at a concentrationof 200 µM, 1.5 mM MgCl₂, 20 ng of bovine serum albumin, 5 µl of10× PCR buffer (100 mM Tris-HCl [pH 9], 500 mM KCl), and 2.5 Uof Taq DNA polymerase (Boehringer, Mannheim, Germany) was adjustedto a final volume of 50 µl with sterile water (Sigma) and overlaidwith 3 drops of mineral oil (Sigma). The tubes were incubatedfor 3 min at 94°C and then subjected to 25 cycles consisting ofdenaturation at 94°C for 1 min, annealing at 55°C for 1 min, andprimer extension at 72°C for 2 min. The tubes were then incubatedfor 10 min at 72°C.

The PCR amplification procedure used for the DGGE analysis was performed with a Perkin-Elmer model 480 thermal cycler. Theconcentrations of chemicals and the quantity of template DNA werethe same as those described above. The tubes were first incubatedfor 5 min at 94°C. A touchdown PCR (12) was then performed byusing 20 cycles consisting of denaturation at 94°C for 1 min,annealing at 65°C (the temperature was decreased by 1°C everysecond cycle until the touchdown temperature of 56°C was reached)for 1 min, and primer extension at 72°C for 1 min. Five additionalcycles were carried out at an annealing temperature of 55°C. Thetubes were then incubated for 10 min at 72°C.

Aliquots (4 µl) of the amplification products were analyzed first by electrophoresis in 1% (wt/vol) agarose gels and thenby ethidium bromide staining. DNA isolation, preparation of PCRmixtures, and pipetting of template DNA into PCR tubes were performedin UV-treated hoods in separate rooms in order to avoid contaminationof the PCR reagents. Different pipettes fitted with autoclavedfilter tips were used in each hood.

DGGE analysis. The PCR products obtained with primers GM5F-GC-clamp and 518R were analyzed by DGGE. DGGE was performed with a Bio-Rad ProteanII system or a Ingeny system as described previously (47, 48).PCR samples were applied directly onto 8% (wt/vol) polyacrylamidegels in 0.5× TAE (20 mM Tris-acetate [pH 7.4], 10 mM acetate,0.5 mM disodium EDTA). The denaturing gradients contained 30 to70% denaturant (100% denaturant corresponded to 7 M urea and 40%[vol/vol] formamide). The gels were prepared with a Minipuls-2pump (Gilson) and a gradient former. Electrophoresis was performedfor 16 h at 75 V and 25 mA (Bio-Rad Protean II system) or at 100V and 25 mA (Ingeny system). The temperature was set at 60°C.After electrophoresis, the gels were incubated for 30 min in watercontaining 0.5 mg of ethidium bromide per liter and photographedon a Mini-Transilluminator UV table equipped with a digital camera(Imager 2.03 system; Appligene Inc.).

After the DGGE analysis of the individual biofilm samples, the individual DGGE profiles were compared to each other by usingthe pairwise similarity coefficient C_s, which was determined asfollows: C_s = 2j/(a + b) × 100, where a was the number of DGGEbands in biofilm 1, b was the number of DGGE bands in biofilm2, and j was the number of common DGGE bands (46, 50). Twoidentical DGGE profiles had a C_s value of 100%, and two completelydifferent profiles had a C_s value of 0%.

Cloning. PCR products obtained with primers 27F and 1492R were purified with a Wizard DNA Clean-Up system (Promega) and cloned by theTA cloning method in pCR2.1 vectors (DNA from freeze-thawed biofilms)and pGemT vectors (DNA from bead-beaten biofilms) with TA cloningkits (Invitrogen and Promega, respectively). Ligation with T4DNA ligase and transformation with One Shot competent cells wereperformed by using the protocols recommended by the manufacturer.Recombinants which were white when they were plated onto X-Gal(5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside)-IPTG (isopropyl- $beta$ -D-thiogalactopyranoside)indicator plates (20 µg of X-Gal per liter, 5 µg of IPTG per liter)were picked and grown overnight in liquid medium (Luria-Bertanibroth). Luria-Bertani broth and indicator plates also containedampicillin (20 µg/liter) and methicillin (80 µg/liter). For thePCR, 1 µl of each clone culture was used directly as a DNA templatewith primers GM5F-GC-clamp and 518R. The PCR conditions were thesame as those described above for the DGGE analysis. The PCR productswere used in a DGGE as described above. Clones that produced aDGGE band at the same position as a band in the environmentalprofiles were partially sequenced (the environmental profileswere the DGGE profiles of the pooled biofilm samples). For sequencing,plasmids were isolated and purified from each clone culture witha High Pure plasmid isolation kit (Boehringer).

Sequencing methods. Cycle sequence reactions were performed with the plasmid-cloned material by using Thermosequenase (Amersham, Little Chalfont,United Kingdom) according to the manufacturer's instructions.Fragment separation, detection, and base calling were performedwith a Vistra model 725 automatic sequencer (Amersham). The sequenceswere determined in one direction with primer 1053-Tex, which isspecific for the domain Bacteria (19), labelled with Texas Red.The sequence of the sequencing primer is shown in Table 1.

Sequence analysis. The sequences obtained were compared to known sequences by using Mail-FASTA program, version GCG73 (53), and the SIMILARITY_RANKtool of the Ribosomal Database Project (RDP) (41), last updatedon 17 May 1995. The sequences were checked for chimeric moleculesby using the CHECK_CHIMERA tool of the RDP. Nucleotide sequencesof close evolutionary relatives of our sequences were retrievedfrom the National Center for Biotechnology Information World WideWeb ENTREZ browser that maintains and distributes the GenBanksequence database. Sequences were aligned manually with the sequencealignment editor SeqApp (Macintosh version 1.9a) (26). Phylogenetictrees were constructed with programs of the PHYLIP program package(Macintosh version 3.5c) (18). For the distance matrix methodwe used DNADIST with the Jukes-Cantor model; phylogenetic treeswere then constructed from evolutionary distances by the neighbor-joiningmethod implemented through the program NEIGHBOR. For the parsimonyand maximum-likelihood methods we used the programs DNAPARS andDNAML (under the default settings) implemented in the PHYLIP softwarepackage. A total of 100 bootstrapped replicate resampling datasets were generated with SEQBOOT. The bootstrap values indicatethe resampling percentages which supported a specific branchingpattern. The consensus tree was determined with CONSENSE. Thesimilarity values given in the test (S) are noncorrected distancesthat were calculated from corrected-distance DNADIST matricesby reversing the Jukes-Cantor corrected distance formulae (35).

The 16S rRNA sequences of the following organisms were used in this study (the numbers in parentheses are GenBank nucleotidesequence accession numbers): Pseudoalteromonas atlantica (X82134),Pseudoalteromonas aurantia (X82135), Pseudoalteromonas carrageenovora(X82136), Pseudoalteromonas citrea (X82137), Pseudoalteromonasdenitrificans (X82138), Pseudoalteromonas espejiana (X82143),Pseudoalteromonas haloplanktis subsp. haloplanktis (X67024),P. haloplanktis subsp. tetraodonis (X82139), Pseudoalteromonasluteoviolacea (X82144), Pseudoalteromonas nigricifaciens (X82146),Pseudoalteromonas piscida (X82141), Pseudoalteromonas rubra(X82147), Pseudoalteromonas undina (X82140), Beggiatoa alba(L40994), clone PVB_OTU_4 (U15116), Colwellia psychroerythrus(L10939), isolate SCB11 (Z31658), marine clone agg53 (L10950),Oceanospirillum linum (M22365), Pseudomonas aeruginosa (M34133),Sphaerotilus natans (Z18534), strain S51-W(gv)1 (U14581),Teredinibacter turnerae (M64339), Thiothrix nivea (L40993),Thiothrix ramosa (U32940), "Antarcticum vesiculatum" (M61002),Cytophaga flevensis (M58767), Cytophaga lytica (M62796),Flavobacterium odoratum (M58777), Flectobacillus glomeratus(M58775), Flexibacter canadensis (M62793), Flexibacter maritimusN⁰449, NCIMB 2154 (D14023), F. maritimus ATCC 43398 (M64629),F. maritimus JCM 8137 (D12667), and isolate 301 (U14586).

Nucleotide sequence accession numbers. The sequences obtained in this study have been assigned in the GenBank database under accession no. AF017792 to AF017805.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

DGGE analysis of the pooled biofilm DNA samples. The two sets of equal-size 16S rDNA PCR products, samples E1 and E2, produced two different DGGE profiles (Fig. 1). The totalnumbers of bands detected in the profiles were 25 for sample E1and 11 for sample E2. Replicates produced the same numbers ofbands (data not shown). The profiles contained intense DNA bands,as well as faint DNA bands. Ten bands, including three intensebands, were found in both profiles.

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FIG. 1. (a) Negative image of ethidium bromide-stained DGGE gels. Lanes E1 and E2, DGGE profiles of pooled biofilm samples E1 (freeze-thaw extraction) and E2 (bead-beating extraction), respectively; lanes 1 to 20, DGGE profiles of 20 individual biofilm samples. (b) Graphic representation of the DGGE profiles shown in panel a. Column C indicates the clones obtained from the three screenings. Columns E1 and E2 indicate the bands produced by pooled biofilm samples E1 and E2, respectively (black DGGE bands represent intense bands). The Filaments line indicates the presence of Beggiatoales-like filamentous bacteria (0, no filaments; $-$ , few filaments; +, abundant filaments). Column H, indicates the number of individual biofilm samples which produced each band. Column N indicates DGGE position. The Size (mm) line indicates the lengths (anteroposterior axis) of the bivalves (in millimeters). Line V indicates the number of bands produced by each sample or (for column C) the number of clones. Columns 1 to 20 show the DGGE profiles of the 20 individual biofilm samples.

DGGE analysis of the individual biofilm DNA samples. Twenty individual biofilms were analyzed by DGGE. Each biofilm produced a different DGGE pattern containing intense and faintbands (Fig. 1). Each pattern was reproducible (data not shown).The number of individual bands varied from 9 to 21. Figure 1bshows that the DGGE profiles were independent of the size of thebivalve and that no particular profile occurred when Beggiatoales-likebacteria were present. Two biofilm samples (biofilm samples 7and 15) produced no DGGE profiles; this may have been due to thepoor development of these biofilms. When the 18 other DGGE profileswere examined, a total of 40 different bands were found. One band(band N27) was present in all of the biofilm samples examined;seven bands (bands N12, N14, N19, N24, N27, N33, and N34) werepresent in at least 15 biofilms; two bands (bands N9 and N22)were present in more than 10 but less than 15 biofilms; and eightbands (bands N5, N6, N8, N10, N15, N18, N37, and N40) were presentin more than 5 but less than 10 biofilms. The most frequent bandin the individual biofilm DGGE patterns (band N27) was probablyan artifact due to fortuitous contamination by Escherichia coliDNA (band N27 migrated to the same position on DGGE gels as theband originating from E. coli 16S rRNA, and a faint band was alsofound at this position in the negative controls). As PCR amplificationswere performed with the greatest care (see above), this contaminationmay have originated from the E. coli used during industrial productionof the Taq enzyme.

The 18 DGGE profiles were compared to one another by using the similarity coefficient C_s (Table 2) without taking band N27into account. The C_s values ranged from 32 to 84%, and the meanC_s value was 54%. The highest C_s values (C_s values greater than75%) were always obtained for biofilm profiles originating frombivalves living in the same burrow; for example, the C_s valuefor biofilms 1 and 2 was 78%, the C_s value for biofilms 10 and11 was 80%, and the C_s value for biofilms 16 and 17 was 84%. Thedata in Table 2 show that the mean intraburrow C_s values (calculatedwith the bold-faced C_s values in Table 2) were not significantlyhigher than the mean interburrow C_s values (calculated withoutthe bold-faced C_s values in Table 2) (except for burrows B1 andB6, which contained only two bivalves).

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TABLE 2. C_s matrix for individual biofilm samples^a

Cloning and sequencing. Three DNA libraries were obtained; these libraries were designated libraries I, II, and III (the freeze-thaw DNA extractionmethod was used for libraries I and II, and the bead-beating DNAextraction method was used for library III). Twenty clones werepicked from library I (S1 clones), 25 clones were picked fromlibrary II (S2 clones), and 17 clones were picked from libraryIII (S3 clones). The S1 clones produced 9 different bands on DGGEgels, the S2 clones produced 8 different bands, and the S3 clonesproduced 10 different bands. The number of clones obtained ateach DGGE position and the clones that were sequenced are indicatedin Fig. 2. No S2 clones were sequenced (the bands were representedin the S1 clones or were not abundant). Only seven of the eightS1 clones sequenced produced a readable sequence (in which basepeaks were well resolved) containing ca. 600 nucleotides; theS1C36 sequence was not readable. The nine S3 clones that weresequenced produced nine readable sequences containing ca. 500nucleotides.

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FIG. 2. Graphic representation of the DGGE profiles obtained from the three screenings. Column N indicates DGGE position. Columns S1, S2, and S3 indicate the bands obtained from the first (S1), second (S2), and third (S3) screenings. The numbers between the columns indicate the numbers of clones obtained for each DGGE position.

Sequence analysis. The 16 readable sequences obtained were submitted to the CHECK_CHIMERA service of the RDP. Two sequences (sequences S1C9 andS1C29) exhibited classic chimeric behavior; the CHECK_CHIMERAhistogram values consistently rose and fell (the histogram forS1C29 was somewhat irregular), and the maximum oligo-gain valueswere high (about 40). Moreover, the S_ab values for the full-lengthsequences were lower than the S_ab values for the fragments. Inaddition, S1C9 was not found in the individual DGGE patterns (Fig.1b). Two other sequences (sequences S1C26 and S1C35) were moreproblematic because they did not exhibit typical chimeric behavior;the histograms rose slowly and irregularly toward moderate oligo-gainvalues (about 25 and 19, respectively), and only S1C26 had a full-lengthsequence S_ab value lower than the S_ab values of the fragments.Many biofilms produced bands corresponding to sequences S1C26and S1C35 in their DGGE patterns (Fig. 1b). These sequences couldrepresent a novel lineage of the domain Bacteria because theypossess all of the signature nucleotides and do not group withany of the lineages of that domain (data not shown). Before definiteconclusions are made, clones S1C26 and S1C35 should be sequencedcompletely.

The 12 sequences for which there was no indication of chimerism were aligned with the sequences of close relatives and usedto construct phylogenetic trees. The 16S rRNA region at E. colibase positions 508 to 991 (length, 484 nucleotides) was utilizedin the analysis. This region spans the V5 hypervariable regionof the 16S rRNA molecule (49). None of the sequences was identicalto any of the known sequences obtained from the databases examined.The sequences fell into two major lineages of the domain Bacteria(51): the $gamma$ -Proteobacteria lineage (nine sequences) and theCytophaga-Flavobacter-Bacteroides lineage (three sequences). Withinthe $gamma$ -Proteobacteria lineage, none of our sequences grouped withthe Beggiatoales. All groups were identified by the three methodsof phylogenetic analysis used and were supported by high bootstrapreplication values. The phylogenetic trees obtained from the distancematrix analysis are shown in Fig. 3 to 5.

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FIG. 3. Phylogenetic tree showing the relationship between the Pseudoalteromonas-related 16S rDNA clones and Pseudoalteromonas species. All of the bacteria are members of the $gamma$ Proteobacteria. P. denitrificans served as the outgroup. The tree was generated by the distance matrix method. The numbers are the bootstrap values for the nodes, based on a total of 100 replicate resamplings (values less than 50 are not shown). The horizontal dotted lines do not represent phylogenetic distances. The nonpigmented Pseudoalteromonas species are surrounded with a dashed square. Bar = 1% nucleotide change. P., Pseudoalteromonas; P. hal. haloplanktis, P. haloplanktis subsp. haloplanktis; P. hal. tetraodonis, P. haloplanktis subsp. tetraodonis.

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FIG. 4. Phylogenetic tree showing the relationship between the 16S rDNA clones related to C. psychroerythrus, O. linum, and PVB_OTU_4 and related bacteria. All of the organisms are members of the $gamma$ Proteobacteria. S. natans served as the outgroup. The tree was generated by the distance matrix method. The numbers are bootstrap values for the nodes, based on a total of 100 replicate resamplings (values less than 50 are not shown). Bar = 5% nucleotide change. B., Beggiatoa; C., Colwellia; O., Oceanospirillum; P., Pseudomonas; T., Teredinibacter; Thx., Thiothrix; S., Sphaerotilus.

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FIG. 5. Phylogenetic tree showing the relationship between the 16S rDNA clones related to the genus Flexibacter and related bacteria. All of the organisms are members of the Cytophaga-Flavobacter-Bacteroides phylum. F. canadensis served as the outgroup. The tree was generated by the distance matrix method. The numbers are bootstrap values for the nodes, based on a total of 100 replicate resamplings (values less than 50 are not shown). Bar = 5% nucleotide change. A., Antarcticum; Cy., Cytophaga; F., Flavobacterium; Flc., Flectobacillus; Flx., Flexibacter.

$gamma$ -Proteobacteria-related sequences. Sequences S3C7, S3C8, S3C13, and S3C14 were members of the $gamma$ 3 subgroup. These sequences grouped with the robust monophyletictaxon which includes the 12 Pseudoalteromonas (formerly Alteromonas)species (23) (Fig. 3). More precisely, these four sequencesgrouped with the nonpigmented Pseudoalteromonas species. The 16SrRNA region examined here was shorter; a total of 390 positions(corresponding to E. coli positions 608 to 991), including bothconserved and hypervariable domains, were included in the analysis.The four Pseudoalteromonas-related sequences differed at six positions(mutations) and by 10 deletion-insertion events in the regionexamined, so the existence of this set of related sequences isnot artifactual (the highest error rate reported for Taq was aboutone mistake per 364 nucleotides [14]). Moreover, the E. coliclones corresponding to sequences S3C7, S3C8, S3C13, and S3C14produced different bands on DGGE gels; this indicates that thesequences did not result from a sequencing artifact. The foursequences were also represented by different bands in environmentalDGGE profiles, so the sequence differences were probably not theresult of mutations during amplification of the plasmids by cloning.

Sequences S1C12, S1C20, and S3C15 were related to the Colwellia cluster. This group includes the psychrophilic marine bacteriumC. psychroerythrus (10), gas vacuolate Antarctic strain S51-W(gv)1(31), and clone AGG 53 (9) (Fig. 4). Sequence S1C18 was relatedto the bacteria O. linum and T. turnerae (11) (Fig. 4). S3C16was related to the hydrothermal vent bacterium clone PVB_OTU_4(44) (Fig. 4).

Cytophaga-Flavobacter-Bacteroides-related sequences. Se- quences S3C18, S3C19, and S3C20 grouped together in the F. maritimus cluster of the Cytophaga subgroup (24) and, moreprecisely, with three F. maritimus strains, NCIMB 2154, JCM 8137,and ATCC 43398 (Fig. 5) (in the region examined, ATCC 43398 andNCIMB 2154 differed by only one nucleotide, and ATCC 43398 andJCM 8137 differed by four nucleotides). F. maritimus is the sameorganism as Cytophaga marina, but the name F. maritimus has priority(34). Like the Pseudoalteromonas-related sequences, the threeF. maritimus-related sequences also represented a set of phylogeneticallyrelated organisms.

Except for DGGE band N27, which is an E. coli band, it appears from Fig. 1b that the most abundant DGGE bands in the individualbiofilm patterns corresponded to Pseudoalteromonas-related sequenceS3C7 (found in 17 of 18 bivalves), Colwellia-related sequenceS3C15 (15 bivalves), and F. maritimus-related sequence S3C20 (15bivalves). The DGGE bands obtained with the Oceanospirillum strainand PVB_OTU_4 appeared less frequently (seven bivalves and onebivalve, respectively). Three other bands were observed frequentlyin the patterns; two were not cloned (DGGE bands N33 and N34)(15 bivalves), and the third was the S1C35 band (17 bivalves),a sequence that could represent a novel lineage of the domainBacteria. There were no clear relationships between the presenceof Beggiatoales-like bacteria in the biofilm and a particularclone.

Sequence signature analysis. The 12 sequences were checked for the presence of signature nucleotides in the 16S rDNA region examined. A total of 23 positionswere examined for the $gamma$ -Proteobacteria lineage (74), and 21positions were examined for the Cytophaga-Flavobacter-Bacteroideslineage (24). The signatures of our sequences were consistentwith the phylogenetic placement of the sequences. There was onlyone difference between the S1C20, S1C12, S3C15, and S1C18 sequencesand the $gamma$ -Proteobacteria consensus sequence (G instead of A atposition 640). In this case, a compensatory base change alwaysoccurred at position 598 (positions 640 and 598 formed a basepair in the 16S rRNA secondary structure). Two positions differedin all of the Pseudoalteromonas and Pseudoalteromonas-relatedsequences (G instead of A at position 640; T instead of G at position760). The following three positions differed in S3C16: position554 (T instead of A), position 690 (A instead of G), and position812 (C instead of G) (the same differences occurred in the closeevolutionary relative PVB_OTU_4). The three Cytophaga-Flavobacter-Bacteroidessequences contained all of the sequence signatures that characterizedthe F. maritimus cluster of the Cytophaga subgroup (24).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

DGGE analysis. We concluded from our DGGE analyses that the biofilms studied were not monospecific; the individual biofilms on average produced13 DGGE bands. Muyzer and de Waal found that the number of DGGEbands in a pattern is related to the number of bacterial speciesin the community (47). Although heteroduplex formation (20)and possible divergence within multicopy rRNA gene families (67)might increase the number of DGGE bands, many other factors shouldreduce it, including sampling biases, differential DNA extraction(61), PCR biases (59), and comigration on DGGE gels (46).To summarize, we view the biofilms studied as complex microecosystemscontaining at least 13 microorganisms belonging to the domainBacteria. The influence of the DNA extraction protocol on thenumber of DGGE bands was obvious in this study; the freeze-thawextraction method (sample E1) was more efficient than the bead-beatingextraction method (sample E2). The complexity of the M. ferruginosabiofilm is not surprising because it was suggested previouslyby microscopic observations (28). In addition, many other studiesof microbial communities have revealed complex consortia (4,21, 32, 60). The fact that there was no apparent relationshipbetween the size (age) of a bivalve and the number of bands inthe DGGE pattern of its biofilm indicates that the complexityof the biofilm cannot be easily related to time. This can be explainedby the biology of the bivalve; the shell, whatever its size, actsas a colonizing area for the microorganisms present in the immediateenvironment (i.e., microorganisms from the sediments, from seaurchin feces, and from other bivalves sharing the same burrow).The immediate environments are not identical for all of the bivalvesliving in the same area. Moreover, as bivalves are active burrowers,their biofilms are frequently abraded; this, along with the heterogeneityof the medium, results in differences among biofilms. On the otherhand, M. ferruginosa is gregarious, and juveniles often attachto adults. This behavior may result in progressive homogenizationof the biofilms in a burrow (although the error of the analysiswas too great to be conclusive, the highest C_s values were obtainedfor biofilms originating from the same burrow). These phenomena(abrasion and homogenization) should be independent of the ageof the bivalves.

It appears from our DGGE analyses that each biofilm is unique, because all of the individual DGGE profiles were different.However, some DGGE bands (bands N9, N12, N14, N19, N24, N33, andN34) were found in most of the DGGE profiles. These bands couldrepresent common biofilm bacteria. The other bands may representatypical biofilm bacteria. The presence of atypical bacteria ina biofilm is not surprising if the heterogeneity and high bacterialdiversity of coastal marine sediments are considered (32). Anotherpossibility is that the atypical DGGE bands represent common butless abundant 16S rRNA sequences and that these sequences aremore influenced by PCR biases than the common and abundant sequences(for example, positively charged iron colloids, which are probablypresent in DNA samples, could inhibit amplification of the lessabundant sequences by adsorption).

It should be noted that an intense DGGE band does not necessarily mean that the corresponding bacteria are abundant in thebiofilm because band intensities are also influenced by 16S rRNAgene copy numbers (17), by differential DNA extraction (61),by PCR biases (59, 68), by comigration of two or more sequencetypes (46), or by a combination of these events. Therefore,the in vivo abundance of a sequence type must be confirmed byother methods, such as in situ hybridization.

Cloning and sequence analysis. The following two sets of related sequences were identified in this study: four Pseudoalteromonas-related sequences and threeF. maritimus-related sequences. Sets of phylogenetically relatedbacterial populations that coexist in relatively well-circumscribedmicroecosystems have also been observed in other environments(2, 19, 21, 29, 40, 63). The significance of thisapparently frequent phenomenon is uncertain; it could be the resultof microevolutionary divergence within a multicopy rRNA gene familyor the result of microgeographical adaptation as a result of selection(29, 43, 67).

Since it is thought that major metabolic traits are shared by (phylogenetically) closely related species (52, 69, 74),we can tentatively infer the major metabolic traits of our unknownorganisms by looking at their close evolutionary relatives. Sucha phenotypic inference method reveals the potential metabolictraits of unknown organisms without the necessity of cultivation.If confirmation is needed, suggested traits may direct the designof subsequent research.

Although there are no rules for relating taxonomic units to 16S rRNA similarities, the high levels of similarity (S = 98.2to 99.8%) between four of our sequences and the sequences of thenonpigmented Pseudoalteromonas species suggest that our sequencesrepresent new species or subspecies belonging to the genus Pseudoalteromonas.Pseudoalteromonas species are widely distributed and frequentlyisolated from marine environments (1); these bacteria are strictlyaerobic chemoorganotrophs (23). Interestingly, Pseudoalteromonasstrains are known to produce siderophores with an exceptionallyhigh affinity constant for ferric ion (57, 58). As suggestedby Dahanayake and Krumbein (6), siderophore-producing bacteriacould produce various iron minerals, depending on the microenvironmentalredox conditions. Also interesting are the high levels of similarity(S = 99.5 to 99.8%) between our sequences and the sequence ofP. haloplanktis subsp. tetraodonis. This organism, like a numberof other marine bacteria, produces tetrodotoxin, a strong neurotoxinthat is the cause of pufferfish poisoning. Such bacteria, whichare frequently encountered in seawater and are associated withmarine animals (64, 65), could protect the microbial communityfrom biofilm grazers.

The close relatives of sequences S1C12 and S1C20 (Colwellia group) and sequence S1C18 (Teredinibacter-Oceanospirillum group),as well as sequences S3C18, S3C19, and S3C20 (F. maritimus group),are aerobic chemoorganotrophs that were found to be symbiotic;C. psychroerythrus was isolated from the surface of flounder eggs(7), T. turnerae was isolated from the gland of Deshayes inshipworms (Bivalvia, Teredenidae) (11, 72), and F. maritimusis epibiotic on marine fishes (70). The similarity values rangedfrom 93.4 to 99.0%. O. linum is not known to be symbiotic; itwas isolated from coastal seawater. A strain related to the genusOceanospirillum has been reported to be able to oxidize manganese(15). If this metal-oxidizing ability is present, the organismrepresented by S1C18 could contribute to iron deposition withinbiofilms (25).

S3C16 grouped with the PVB_OTU_4 sequence (S = 93.2%). The latter sequence was retrieved from the bacterial mat communityof Pele's Vents, an active deep-sea hydrothermal vent system inHawaii (44). The exact phylogenetic placement of PVB_OTU_4 isstill uncertain; the corresponding bacterium is probably chemolithoautotrophic(44). It is worth noting that bacterial mats collected fromthis vent system are made up of long filaments coated with amorphousiron precipitates rich in Ca and P (36, 37), like the biofilmcovering M. ferruginosa (28). The vent field bacterial mats,which are apparently dominated by Thiovulum-related species andXanthomonas-related species, also contain bacteria related tothe genera Colwellia (sequence PVB 54) and Alteromonas (Pseudoalteromonas)(sequence PVB 18), like the biofilm in the present study. It isnot known if there is any relationship between the simultaneouspresence of these three sequences (sequences related to PVB_OTU_4,Colwellia, and Pseudoalteromonas) and the presence of an amorphousiron mineral deposit rich in P and Ca. If S3C16 represents a chemolithoautotrophicbacterium, this bacterium could participate in the formation ofthe iron deposit (by contributing an iron-oxidizing activity).However, the organism represented by sequence S3C16 probably doesnot occur frequently in the M. ferruginosa biofilm (Fig. 1b).

The epibiotic bacteria may have several effects on the biology of M. ferruginosa. Most of our sequences were related to thesequences of epibiotic chemoorganotrophic marine bacteria. Thepresence of such bacteria on the bivalve (we suppose that we mayinfer that this type of metabolism occurs with some confidence),which produces various hydrolytic enzymes, can be problematic;these bacteria could degrade the periostracum of the mollusk (theouter layer of mollusk shells is composed of a scleroprotein calledconchiolin), as well as the organic shell matrix (which is richin glycoproteins, polypeptides, and polysaccharides) (66). Actually,proteolytic and chitinase-producing microorganisms, like C. psychroerythrusand probably the organisms represented by our related sequences,have been found in degrading mollusk shells (56). This couldexplain why many M. ferruginosa have highly degraded shells undertheir biofilms (unpublished data). The epibiotic bacteria couldalso provide benefits to the bivalve by immobilizing toxic ironions and sulfide (28) and by producing toxic compounds, suchas tetrodotoxin. The chemoorganotrophic metabolism could alsobe related to iron deposition because most of the iron in seawateris probably complexed by organic ligands (30), and microbialdegradation of these ligands could lead to subsequent depositionof ferric minerals (16).

In future studies we will determine the in vivo abundance of our sequences with general and specific oligodeoxynucleotideprobes. We also plan to study the M. ferruginosa biofilm withcultivation techniques and to test the probes on the cultures.We hope that this integrated approach will lead to a better understandingof the roles of microorganisms in the processes of mineral depositionwithin the M. ferruginosa biofilm.

	ACKNOWLEDGMENTS

We thank all of the members of the Department of Microbial Ecology for their friendly help and Steve Nold for his commentson the manuscript.

This work was supported by FRIA grant 940733 to D.C.G and by FRFC grant 2-4510-96 to C.D.R.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire de Biologie Marine, CP 160/15, Université Libre de Bruxelles, 50 av. Roosevelt,1050 Brussels, Belgium. Phone: 32-2-6502970. Fax: 32-2-6502796.E-mail: dgillan{at}ulb.ac.be.

A contribution of the Centre Interuniversitaire de Biologie Marine.

REFERENCES

Top
Abstract
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Materials & Methods
Results
Discussion
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