Impact of Culture-Independent Studies on the Emerging Phylogenetic View of Bacterial Diversity

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Journal of Bacteriology, September 1998, p. 4765-4774, Vol. 180, No. 18
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

MINIREVIEW
Impact of Culture-Independent Studies on the Emerging Phylogenetic View of Bacterial Diversity

Philip Hugenholtz, Brett M. Goebel, and Norman R. Pace^*

Departments of Plant and Microbial Biology and Molecular and Cell Biology, University of California, Berkeley, Berkeley, California 94720-3102

	INTRODUCTION

Top Introduction Conclusion References

Our perspective on microbial diversity has improved enormously over the past few decades. In large part this has been dueto molecular phylogenetic studies that objectively relate organisms.Phylogenetic trees based on gene sequences are maps with whichto articulate the elusive concept of biodiversity. Thus, comparativeanalyses of small-subunit rRNA (16S or 18S rRNA) and other genesequences show that life falls into three primary domains, Bacteria,Eucarya, and Archaea (51, 52). Based on rRNA trees, the mainextent of Earth's biodiversity is microbial. Our knowledge ofthe extent and character of microbial diversity has been limited,however, by reliance on the study of cultivated microorganisms.It is estimated that >99% of microorganisms observable in naturetypically are not cultivated by using standard techniques (1).

Recombinant DNA and molecular phylogenetic methods have recently provided means for identifying the types of organisms thatoccur in microbial communities without the need for cultivation(see references 1, 20, and 35 for reviews). Results fromapplication of these methods to a number of diverse environmentsconfirm that our view of microbial diversity was limited and pointto a wealth of novel and environmentally important diversity yetto be studied (34). It is the aim of this review to collate,compare, and incorporate the results of the environmental sequence-basedstudies into the context of known bacterial diversity. We discussthe sequence data at the taxonomic level of the phylogenetic divisionbecause divisions constitute first-order clades for describingthe breadth of bacterial diversity. Although we have yet to determineeven the outlines of the bacterial tree, common threads are beginningto emerge that revise our current views of bacterial diversityand distribution in the environment.

	PHYLOGENETIC DIVERSITY IN THE BACTERIAL DOMAIN

In 1987, Woese described the bacterial domain as comprised of about 12 natural relatedness groups, based mainly on analysesof familiar cultivated organisms such as cyanobacteria, spirochetes,and gram-positive bacteria (all of which, based on rRNA sequencedivergence, display greater evolutionary depth than plants, animals,and fungi) (51). These relatedness groups have variously beencalled "kingdoms," "phyla," and "divisions"; we use the latterterm. For the purposes of this review we define a bacterial divisionpurely on phylogenetic grounds as a lineage consisting of twoor more 16S rRNA sequences that are reproducibly monophyleticand unaffiliated with all other division-level relatedness groupsthat constitute the bacterial domain. We judge reproducibilityby the use of multiple tree-building algorithms, bootstrap analysis,and varying the composition and size of data sets used for phylogeneticanalyses. The typical interdivisional rRNA sequence differenceis 20 to 25%. For comparison, the 16S rRNAs of Escherichia coliand Pseudomonas aeruginosa, both representatives of the $gamma$ groupof Proteobacteria, differ overall by about 15%; the 16S rRNAsof E. coli and Bacillus subtilis ("low-G+C gram-positive bacterial"division) differ by about 23%.

At the current stage in the phylogenetic classification of Bacteria, divisions are not consistently named or taxonomicallyranked. rRNA-defined divisions are identified by classes (e.g.,Proteobacteria [41] and Actinobacteria [42]), orders (e.g.,Thermotogales and Aquificales), families (e.g., Chlorobiaceae),generic names such as the Nitrospira group (11), or common namessuch as the green nonsulfur (GNS) bacteria and low-G+C gram-positivebacteria (51). Division-level nomenclature has not even beenconsistent between studies, so some divisions are identified bymore than one name. For instance, green sulfur bacteria is synonymouswith Chlorobiaceae; high-G+C gram-positive bacteria is synonymouswith Actinobacteria and Actinomycetales. Indeed, it probably ispremature to standardize taxonomic rankings for bacterial divisionsat this point when our picture of microbial diversity is likelystill incomplete and the topology of the bacterial tree is stillunresolved.

In the past decade the number of identifiable bacterial divisions has more than tripled to about 40 due in significant partto culture-independent phylogenetic surveys of environmental microbialcommunities (21, 34). These analyses rely on sequences ofrRNA genes obtained by cloning directly from environmental DNAor, as in the majority of studies, after amplification by thePCR (1, 20, 35). Figure 1 represents the division-leveldiversity of the bacterial domain as inferred from representativesof the approximately 8,000 bacterial 16S rRNA gene sequences currentlyavailable. Although 36 divisions are shown in Fig. 1, severalother division-level lineages are indicated by single environmentalsequences (9, 21, 37), suggesting that the number of bacterialdivisions may be well over 40. Several of the described divisionsare well represented by cultivated strains and were the firstto be characterized phylogenetically (51). The majority of thebacterial divisions, however, are poorly represented by culturedorganisms. Indeed, 13 of the 36 divisions shown in Fig. 1 arecharacterized only by environmental sequences (shown outlined)and so are termed "candidate divisions" to indicate their unsubstantiatedstatus as new bacterial divisions (21). One of these candidatedivisions, OP11, is now sufficiently well represented by environmentalsequences to conclude that it constitutes a major bacterial group(see below). Phylogenetic studies so far have not resolved branchingorders of the divisions; bacterial diversity is seen as a fan-likeradiation of division-level groups (Fig. 1). The exception tothis, however, is the Aquificales division, which branches mostdeeply in the bacterial tree in most analyses.

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FIG. 1. Evolutionary distance tree of the bacterial domain showing currently recognized divisions and putative (candidate) divisions. The tree was constructed using the ARB software package (with the Lane mask and Olsen rate-corrected neighbor-joining options) and a sequence database modified from the March 1997 ARB database release (43). Division-level groupings of two or more sequences are depicted as wedges. The depth of the wedge reflects the branching depth of the representatives selected for a particular division. Divisions which have cultivated representatives are shown in black; divisions represented only by environmental sequences are shown in outline. The scale bar indicates 0.1 change per nucleotide. The aligned, unmasked data sets used for this figure and Fig. 3 through 6 are available from http://crab2.berkeley.edu/pacelab/176.htm.

	BACTERIAL DIVERSITY AND DISTRIBUTION IN THE ENVIRONMENT

Culture-dependent studies indicate that representatives of some bacterial divisions are cosmopolitan in the environment, whereasothers appear restricted to certain habitats (39). Culture-independentstudies so far conducted reflect and expand this view. Table 1summarizes the environmental distribution of sequences by habitattype, compiled from most of the available 16S rRNA-based clonalanalyses: 86 studies contributing nearly 3,000 sequences. An expandedversion of this table that details division-level representationin the individual studies is available at http://crab2.berkeley.edu/pacelab/176.htm.Table 1 includes only divisions for which representatives havebeen detected in at least two independent studies and for whichat least one near-complete 16S rRNA gene sequence is known. Table1 is, therefore, not an exhaustive listing of potential division-leveldiversity for all studies.

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TABLE 1. Summary of 16S rRNA-based clonal analyses of diversity of uncultivated bacteria^a

Sequence representatives of several bacterial divisions have been identified in a wide range of habitats, suggesting the cosmopolitanor ubiquitous distribution of the corresponding organisms in theenvironment and, potentially, their broad metabolic capabilities.Some of these cosmopolitan divisions are well-known from cultivationstudies; however, others are little known or have not yet beendetected by cultivation. Figure 2 summarizes the representationof selected cosmopolitan divisions by sequences of cultivatedand uncultivated organisms. The Proteobacteria (purple photosyntheticbacteria and relatives), Cytophagales (Bacteroides-Cytophaga-Flexibactergroup), and the two gram-positive divisions, Actinobacteria andlow-G+C gram-positive bacteria, are well represented by cultivatedorganisms and therefore are familiar to us in principle. Thesefour divisions account for 90% of all cultivated bacteria characterizedby 16S rRNA sequences and approximately 70% of the environmentalsequences collated in Table 1. By contrast, other cosmopolitandivisions revealed by clonal analyses, such as Acidobacterium,Verrucomicrobia, GNS bacteria, and OP11, are poorly representedby sequences from cultivated organisms (Fig. 2) and consequentlyare little known with regard to their general properties. Althoughmany of the bacterial divisions occur widely, others seem to occupya more limited range of habitats (Table 1). All cultivated representativesof Aquificales, for instance, are thermophilic hydrogen metabolizers,and all environmental sequences of Aquificales have been obtainedonly from high-temperature environments. This suggests a specializedhabitat niche for this group. Alternatively, the apparently limitedenvironmental distribution may simply reflect a sampling or methodologicalartifact and representatives of such divisions may be presentin a wider range of habitats, but not yet detected.

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FIG. 2. Relative representation in selected cosmopolitan bacterial divisions of 16S rRNA sequences from cultivated and uncultivated organisms. Results were compiled from 5,224 and 2,918 sequences from cultivated and uncultivated organisms, respectively.

The database of environmental rRNA sequences is compromised in resolving some phylogenetic issues by a large number of relativelyshort sequences. More than half of the sequences collated in Table1 are less than 500 nucleotides (nt) long, which represents onlyone-third of the total length of 16S rRNA. This is due to an unfortunatetrend in many environmental studies of sequencing only a portionof the gene in the belief that a few hundred bases of sequencedata is sufficient for phylogenetic purposes. Indeed, 500 nt issufficient for placement if some longer sequence is closely related(>90% identity in homologous nucleotides) to the query sequence.In the case of novel sequences, <85% identical to known sequences,however, <500 nt is usually insufficient comparative informationto place the sequence accurately in a phylogenetic tree and caneven be misleading.

Since all but 4 (40, 46, 49, 50) of the 86 studies collated in Table 1 were conducted using PCR to amplify rDNA fromextracted environmental DNA, the question arises as to whethermolecular analyses accurately reflect the division-level diversitythat occurs in the environment. It is well established that PCR-associatedartifacts such as differential amplification of different rDNAtemplates (36, 44), sensitivity to rRNA gene copy number (12),PCR primer specificity (48), sensitivity to template concentration(6), amplification of contaminant rDNA (45), and formationof chimeric sequences (23) may skew our assessment of microbialdiversity. Most of the studies collated in Table 1, however,analyzed tens to hundreds of clones, so it seems likely that thesestudies have sampled the main types of sequences in the communitiesexamined. We believe, acknowledging the caveats of the methodology,that the clonal analyses collated in Table 1 probably includethe most abundant (metabolically active) bacterial sequence typesin the samples analyzed, likely representing the members of thecommunities that are involved in the principal metabolic activities,such as carbon cycling.

	ABUNDANT BUT LITTLE-KNOWN BACTERIAL DIVISIONS

The rRNA sequence studies of environmental organisms probably identify the abundant organisms in the environments studiedand, therefore, account for the organisms that participate significantlyin the maintenance of the communities. Because of their abundancein the environment, representatives of some poorly studied phylogeneticdivisions are predicted to play significant roles in environmentalchemistry. Examples of such divisions, which because of theirpotential environmental significance merit study, are the Acidobacteriumdivision, the Verrucomicrobia, the GNS bacteria, and candidatedivision OP11.

Acidobacterium division. The Acidobacterium group is a newly recognized bacterial division with only three cultivated representatives: Acidobacteriumcapsulatum (18), Holophaga foetida (26), and Geothrix fermentans(28). Figure 3 is a phylogenetic dendrogram of this group, includingselected environmental representatives. The limited physiologicalinformation known about these organisms provides few clues toproperties that might be general throughout the division. Acidobacteriumis a moderately acidophilic aerobic heterotroph; Holophaga andGeothrix are strict anaerobes that ferment aromatic compoundsand acetate, respectively. The majority of sequences that makeup this division, however, are from environmental clones. At leasteight monophyletic subdivisions in the Acidobacterium group areidentified by phylogenetic analyses (Fig. 3 [24, 29]). Wedefine a subdivision as a lineage comprised of two or more 16SrRNA sequences within a division that are reproducibly monophyleticand unaffiliated with all other representatives of that division.Acidobacterium subdivisions 1, 3, 4, and 6 are well representedby environmental clone sequences from independent studies, yetno cultivated strains are known with the exception of subdivision1, represented by A. capsulatum. The widespread occurrence ofenvironmental sequences belonging to the Acidobacterium division(Table 1) suggests that members of this group are ecologicallysignificant constituents of many ecosystems, particularly soilcommunities. They have been detected in every clonal analysisof soils (with a wide range of chemical properties), as well asin other habitats, including a peat bog, acid mine drainage, acontaminated aquifer, a hot spring, a freshwater lake, and a sampleof the Atlantic ocean from a depth of 1,000 m (Fig. 3). In situsingle-cell analyses with fluorescent hybridization probes specificfor Acidobacterium subdivision 6 small-subunit rRNA indicate thatthis subdivision is morphologically diverse (29), as expectedfor a broad phylogenetic group. Members likely are metabolicallydiverse as well: the depth of phylogenetic diversity (depth ofbranching) in the Acidobacterium division is nearly as great asin the Proteobacteria.

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FIG. 3. Phylogenetic dendrogram of the Acidobacterium division. Names of cultivated organisms are shown in bold. The habitat source of each environmental sequence is indicated before the clone name. GenBank accession numbers are listed parenthetically. Subdivisions (see the text) are indicated by brackets at the right of the tree. Construction of the tree was as described for Fig. 1. The robustness of the topology presented was estimated by bootstrap resampling of independent distance, parsimony, and rate-corrected maximum-likelihood analyses as previously described (2). Distance and parsimony analyses were conducted using test version 4.0d61 of PAUP*, written by David L. Swofford. Branch points supported (bootstrap values of >75%) by most or all phylogenetic analyses are indicated by filled circles; open circles indicate branch points marginally supported (bootstrap values of 50 to 74%) by most or all analyses. Branch points without circles are not resolved (bootstrap values of <50%) as specific groups in different analyses. The scale bar indicates 0.1 change per nucleotide.

Verrucomicrobia. Verrucomicrobia is a newly proposed division of Bacteria (17) represented by a handful of isolates: Verrucomicrobium spinosum(after which the division is named) (47), four Prosthecobacterspecies (17), and three strains of ultramicrobacteria (22).Verrucomicrobia and Prosthecobacter are prosthecate bacteria isolatedfrom freshwater, and the ultramicrobacteria, "dwarf-cell" strainsonly about 0.1 µm³ in volume, were isolated from a soil habitat. All of these isolatespreferentially use sugars as growth substrates. Culture-independentanalyses indicate that the Verrucomicrobia, like members of theAcidobacterium division, are widespread in the environment andabundant, particularly in soils (Table 1). Figure 4 shows a dendrogramof representatives of the Verrucomicrobia. Several monophyleticsubdivisions are seen, only two of which are represented by thecultivated strains. Clone sequences of this division from soilare predominantly from members of the phylogenetically broad subdivisions2 and 3. The abundance of these two groups suggests their ecologicalimportance. For instance, the abundance of one representativeof Verrucomicrobia subdivision 2 (EA25) was estimated by PCR at10⁷ to 10⁸ cells per g of a pasture soil sample, 1 to 10% of the total microbialcontent (25).

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FIG. 4. Phylogenetic dendrogram of the Verrucomicrobia division. Names of cultivated organisms are shown in bold. The habitat source of each environmental sequence is indicated before the clone name. GenBank accession numbers are listed parenthetically. Subdivisions (see the text) are indicated by brackets at the right of the tree. Tree construction and support for branch points was as described for Fig. 1 and 3, respectively. The scale bar indicates 0.1 change per nucleotide.

In our phylogenetic analyses we consistently find that the division Chlamydia is a specific sister group of the Verrucomicrobia.We find no support for the notion (17, 30, 47) of a specificrelatedness of the planctomycetes with the Verrucomicrobia.

GNS bacteria. The GNS bacteria have been recognized as a division-level bacterial group for over a decade (51). Even today, however, thisdivision is still represented by only a few isolates. The culturedrepresentatives have a wide range of phenotypes, from anoxygenicphotosynthesis (Chloroflexus) to thermophilic organotrophy (Thermomicrobium).Figure 5 shows the relatedness groups of GNS bacteria detectedin the environment. It is apparent from the dendrogram that allof the cultivated representatives except the chlorinated hydrocarbon-reducingDehalococcoides ethenogenes (31) are related in subdivision3, together with several clone sequences from a hot spring, arice paddy, and activated sludge (data not shown). By contrast,most of the environmental sequences described to date fall intoa different relatedness group, subdivision 1, with no cultivatedrepresentatives. Considering the wide variety of habitats thathave contributed GNS sequences (Fig. 5; Table 1), particularlyto GNS subdivision 1, members of this division likely play significantroles in the environment.

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FIG. 5. Phylogenetic dendrogram of the GNS division. Names of cultivated organisms are shown in bold. The habitat source of each environmental sequence is indicated before the clone name. GenBank accession numbers are listed parenthetically. Subdivisions (see the text) are indicated by brackets at the right of the tree. Tree construction and support for branch points was as described for Fig. 1 and 3, respectively. The scale bar indicates 0.1 change per nucleotide.

Candidate division OP11. Candidate division OP11 is a recently proposed novel bacterial division for which there is no reported cultivated representative(19, 21). However, several independent clonal studies havereported environmental sequences that together form the OP11 clade.Figure 6 shows a dendrogram of the known environmental sequencerepresentatives of the division, with five subdivisions currentlyidentifiable. OP11 sequences all have highly atypical sequencesignatures for the domain Bacteria (51), and they have low sequenceidentities, only about 80%, to sequences outside the OP11 division.This may be due to higher-than-average mutation rates in OP11rRNAs, as has been suggested for other groups such as the planctomycetes(27). OP11 sequences have been obtained from a variety of habitatsincluding several different types of soil, freshwater sediments,the deep subsurface, and hot springs (Table 1), suggesting thatmembers of the division play significant ecological roles. Untilcultivated representatives of the OP11 division are characterized,little beyond the general properties of Bacteria can be inferredabout their physiology.

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FIG. 6. Phylogenetic dendrogram of the OP11 division. The habitat source of each environmental sequence is indicated before the clone name. GenBank accession numbers are listed parenthetically. Subdivisions (see the text) are indicated by brackets at the right of the tree. Tree construction and support for branch points was as described for Fig. 1 and 3, respectively. The four MIM clones and F78 clone are unreleased sequences generously made available to us by Pascale Durand (10) and Floyd Dewhirst (8). The scale bar indicates 0.1 change per nucleotide.

Additional candidate divisions. Several additional candidate divisions have been identified based on environmental sequences alone, shown as outlined wedgesin Fig. 1. These divisions comprise two or more sequences over500 nt in length that were obtained mostly from independent studies,or at least from independent PCR events. An expanded view detailingrepresentatives of each candidate division is available at http://crab2.berkeley.edu/pacelab/176.htm.The candidate divisions are identified according to the originalsource or clone names of the sequences that define the clade.Divisions designated OP were originally identified in an analysisof a Yellowstone hot spring, Obsidian Pool (21). Representativesof three of these divisions, OP5, -8, and -10, also have beenencountered in a study of a hydrocarbon-contaminated aquifer atWurtsmith Air Force Base in Michigan (9). The latter studyalso identified novel divisions WS1, now identified in a Siberiantundra soil (53), and WS6. Candidate division marine group Awas originally identified and named based on partial sequencesobtained from marine microbial communities in the Atlantic andPacific oceans (13) and verified by full-length-sequence representativesof the group from similar marine samples (16). Abundance anddepth profiles of marine group A sequences in the water column(16) suggest their global distribution in marine communities;no representatives of this candidate division outside of marineenvironments have yet been obtained (Table 1). Representativesof the termite group I candidate division originally were identifiedas a closely related clade of sequences from the termite gut (33)but now also have been identified in a contaminated aquifer (9).Candidate division OS-K was identified in a study of a Yellowstonehot spring, Octopus Spring (49) and bolstered by additionalrepresentative sequences from studies of a hydrothermal vent (32)and marine sediment (7). Candidate divisions TM6 and TM7 arenamed after sequences obtained in an environmental study of apeat bog (38), and other partial-length-sequence representativesof these candidate divisions were subsequently identified fromactivated sludges (4, 15) and soil (5).

	CONCLUSION

Top Introduction Conclusion References

Phylogenetic trees based on rRNA sequences show that bacterial diversity is represented by natural relatedness groups, thephylogenetic divisions (51). About 36 such divisions are currentlyidentifiable. The final extent of division-level diversity inthe bacterial domain is still unknown but clearly will be morethan 40 divisions. Culture-independent studies have resulted inmultiple hits on the majority of described divisions in differenthabitat types (Table 1), suggesting that the final number ofdivisions will be within the same order of magnitude as the presentestimate.

The molecular analyses of environmental DNA have revealed substantial phylogenetic diversity with little or no representationamong organisms previously studied. Because of their abundanceand wide distribution, some of the organisms represented by thesequences likely contribute significantly to the global chemicalcycles. Descriptions of newly identified, but apparently important,bacterial divisions such as the Acidobacterium and Verrucomicrobia,are presently confounded by too few cultivated representativesand only rudimentary descriptions of the strains. Cultivationefforts need to be directed at new representatives of the diversegroups for further study. Continued work to sequence the 16S rDNAsof all deposited type cultures (<50% sequenced to date [14])may also result in detection of additional cultivated representativesof newly described divisions. It is a challenge to microbial biologiststo determine the physiological diversity and environmental rolesof these recently articulated divisions of Bacteria.

The phylogenetic differences between the bacterial divisions probably are reflected in substantial physiological differences.Some properties, the general properties of Bacteria, are expectedto be distributed among all the divisions. Division-specific noveltiesare known as well, for instance, endospore formation by the low-G+Cgram-positive bacteria or axial filaments (endoflagella) in thespirochetes. Some biochemical properties evidently have transferredlaterally among the divisions. For example, the two types of photosyntheticcomplexes, photosystem I (PSI) and PSII, are each distributedsporadically among the divisions, consistent with lateral transfer(3). Lateral transfer may also have resulted in combinatorialnovelty among the divisions; PSI and PSII, for instance, apparentlycame together in the cyanobacteria to create oxygenic photosynthesis,with profound consequences to the biosphere (3). Many moresuch division-specific qualities and cooperations should becomeevident at the molecular level as comparative genomics gives usa sharper phylogenetic picture of bacterial diversity.

	ACKNOWLEDGMENTS

We thank John A. Fuerst for providing useful comments on the manuscript and Pascale Durand, Floyd Dewhirst, and Bruce Pasterfor supplying unreleased sequences. We also thank Michael Tannerand Scott Dawson for assistance in establishing the website ofadditional information.

The authors' research is supported by grants to N.R.P. from the National Institutes of Health and Department of Energy.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Plant and Microbial Biology, University of California, Berkeley, Berkeley,CA 94720-3102. Phone: (510) 643-2571. Fax: (510) 642-4995. E-mail:nrpace{at}nature.berkeley.edu.

Present address: Australian Magnesium Corporation, Toowong, Queensland, 4066 Australia.

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MINIREVIEW Impact of Culture-Independent Studies on the Emerging Phylogenetic View of Bacterial Diversity

MINIREVIEW
Impact of Culture-Independent Studies on the Emerging Phylogenetic View of Bacterial Diversity