Abstract
In microbial mat communities of Yellowstone hot springs, ribosomal RNA (rRNA) sequence diversity patterns indicate the presence of closely related bacterial populations along environmental gradients of temperature and light. To identify the functional bases for adaptation, we sequenced the genomes of two cyanobacterial (Synechococcus OS-A and OS-B′) isolates representing ecologically distinct populations that dominate at different temperatures and are major primary producers in the mat. There was a marked lack of conserved large-scale gene order between the two Synechococcus genomes, indicative of extensive genomic rearrangements. Comparative genomic analyses showed that the isolates shared a large fraction of their gene content at high identity, yet, differences in phosphate and nitrogen utilization pathways indicated that they have adapted differentially to nutrient fluxes, possibly by the acquisition of genes by lateral gene transfer or their loss in certain populations. Comparisons of the Synechococcus genomes to metagenomic sequences derived from mats where these Synechococcus stains were originally isolated, revealed new facets of microbial diversity. First, Synechococcus populations at the lower temperature regions of the mat showed greater sequence diversity than those at high temperatures, consistent with a greater number of ecologically distinct populations at the lower temperature. Second, we found evidence of a specialized population that is apparently very closely related to Synechococcus OS-B′, but contains genes that function in the uptake of reduced ferrous iron. In situ expression studies demonstrated that these genes are differentially expressed over the diel cycle, with highest expression when the mats are anoxic and iron may be in the reduced state. Genomic information from these mat-specific isolates and metagenomic information can be coupled to detect naturally occurring populations that are associated with different functionalities, not always represented by isolates, but which may nevertheless be important for niche partitioning and the establishment of microbial community structure.
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Introduction
Microbial mats have played a crucial role in the evolution of life on earth, and modern mats are considered to be analogs of the extensive Precambrian microbial communities, which significantly altered the atmosphere and the oxidation/reduction balance of the earth (Hoehler et al., 2001; Teske and Stahl, 2002). Microbial mats thrive in many extreme environments such as hypersaline bays, permanent-ice lakes and hot springs, where competition from other organisms is limited (Paerl et al., 2000). The mats represent model systems for discovering the principles of microbial community ecology and have been studied intensively for decades (Ward et al., 1998, 2006; Stal, 2000).
The dense microbial communities growing in the hot spring effluent channels of Yellowstone National Park are predominantly prokaryotic in nature, affording a unique opportunity to study interactions among different prokaryotes. The mats are relatively stable, simple communities, typical of other mat communities in the sense that organic matter is produced in the uppermost layers by phototrophs and subsequently recycled and used in the deeper layers by aerobic and anaerobic decomposition metabolisms (Ward et al., 1998; Ward and Castenholz, 2000). The mats contain a diversity of microorganisms ranging from phototrophs such as cyanobacteria (predominantly Synechococcus spp.) and green non-sulfur-like bacteria (GNSLB), such as Roseiflexus spp. and Chloroflexus spp., to less well-characterized heterotrophic anaerobic and aerobic bacteria (Brock, 1978; Ward et al., 1998; Ward and Castenholz, 2000). The metabolic activities of and interactions among, the mat-building organisms create impressive stratified structures in which microorganisms may experience steep gradients of light, oxygen and nutrients (Ward et al., 2006).
Early work based primarily on microscopy and cultivation approaches led to the belief that the mat was primarily comprised of a single morphologically recognizable Synechococcus species and that the physical cohesiveness of the mat was provided by the GNSLB, Chloroflexus aurantiacus. With the advent of molecular techniques such as direct sequencing of 16S rRNA from mat clones and denaturing gradient gel electrophoresis (DGGE), it became obvious that the mat contained many unique 16S rRNA sequences, most of which were not identical to the 16S rRNA sequences of isolates cultivated from the mat. Cyanobacterial and GNSLB 16S rRNA sequences detected by molecular analyses were found to be distantly related to those of readily cultivated Synechococcus and Chloroflexus isolates and to occur as sets of closely related sequences differing by <5% in 16S rRNA sequence (Ward et al., 1990; Ferris and Ward, 1997; Nübel et al., 2002). DGGE surveys also revealed that the 16S rRNA gene distributions of the closely related cyanobacterial and GNSLB 16S rRNA populations (we use the term populations to mean sets of related individuals and use adjectives to specify how the individuals within populations are related (for example, cyanobacterial 16S rRNA populations, Synechococcus populations, functionally specialized populations, and so on)) varied along well-defined temperature gradients that exist in the effluent channels. For instance, closely related Synechococcus 16S rRNA sequences designated A″, A′, A, B′ and B, were detected at progressively lower temperatures from about 70°C to about 50°C, respectively (Ferris and Ward, 1997; Ward et al., 1998). Furthermore, recent experiments with Synechococcus isolates representing some of these 16S rRNA sequences suggest that they are physiologically adapted to temperature ranges and light intensities experienced in situ (Allewalt et al., 2006; Kilian et al., 2007). There is also evidence of vertical stratification of Synechococcus populations within the microbial mats. On the basis of fluorescence characteristics and DGGE analysis, physiologically and genetically distinct Synechococcus populations were identified at different depth intervals within the 1-mm thick upper green layer of these mats (Ramsing et al., 2000). Many parameters such as light intensity and quality, UV penetration, oxygen tension, and nutrient fluxes vary as a function of mat depth and over a diel cycle (Ward et al., 2006), although it is not obvious which of these parameters (one or more) lead to the stratification of Synechococcus populations within the mat. This correspondence between sequence variation and microgeographic distribution matches the prediction of some evolutionary ecology models of bacterial speciation, where natural selection acts upon variation to yield distinct phylogenetic clusters of individuals, with each cluster representing an ecologically distinct population (or ‘ecotype’, defined as a clade of individuals related by common ecological characteristics) (Ward, 1998; Ward and Cohan, 2005; Cohan and Perry, 2007). These models provide a framework for using sequence data to discover ecologically distinct populations, which can be considered the fundamental species-like units of which communities are comprised and whose ecological distinctness can be elucidated by genomic and physiological analyses (Cohan, 2006; Ward, 2006; Cohan and Perry, 2007; Ward et al., 2007).
Although a combination of genetic, biochemical and physiological data collected over decades has led to the hypothesis that there may be multiple specialized populations within these stratified mats, the underlying functional and genetic basis for this diversity has not yet been fully appreciated (Ward et al., 1998, 2006). Because the mat Synechococcus populations have been extensively characterized at the level of rRNA diversity and physiology, and are available as isolates, they provide optimal starting material for high-resolution molecular analyses to establish links between physiological differences, niche partitioning strategies and microbial diversity within the mat community (Steunou et al., 2006; Kilian et al., 2007). Here, we present our approach in which we sequenced the genomes of two isolates of Synechococcus derived from different temperature regions of the mat. This analysis has provided us with ‘anchor genomes’ from two differently temperature-adapted Synechococcus isolates whose 16S rRNA sequences correspond to dominant mat sequences, which can be directly compared to each other, and also compared to metagenomic sequences derived from regions of the mat from which these isolates were originally isolated.
Materials and methods
Source of DNA
Synechococcus JA-2-3Aa {genotype designation A-NACy05a} (hereafter Synechococcus OS-A) was isolated by filter cultivation from samples derived from a region of the mat in Octopus Spring exposed to temperatures ranging from 58°C to 65°C; Synechococcus JA-2-3B′a(2-13) {genotype designation B′NACy10o} (hereafter Synechococcus OS-B′) was isolated from Octopus Spring mat samples collected at temperatures ranging from 51 to 61°C (Allewalt et al., 2006). We also generated metagenomic sequences from recombinant libraries from total DNA isolated from the top green layer (upper ∼1 mm) of the microbial mats in Octopus Spring and from Mushroom Spring, a nearby spring with similar physicochemical characteristics (Papke et al., 2003). The samples used to generate the metagenomic sequences were collected from two different temperature-defined sites averaging ∼60 and ∼65°C (Materials and methods and Supplementary Table S5).
Sequencing and annotation of Synechococcus OS-A and OS-B′ genomes
Plasmid libraries with small (2–3 kbp) and large (10–12 kbp) inserts were constructed in pUC-derived vectors following random mechanical shearing (nebulization) of genomic DNA. The plasmid sequences were assembled using the Celera Assembler. The coverage criteria were (a) every position required at least double-clone coverage (or sequence from a PCR product amplified from genomic DNA) and (b) sequences were generated from both strands. The sequence was edited manually, and additional PCR and sequencing reactions were performed to close gaps, improve coverage and resolve sequence ambiguities. Sequences of regions of the DNA that were repeated on the genome were verified by PCR amplification across the repeat followed by sequence analysis of the amplification product. The final assemblies of the Synechococcus OS-A and OS-B′ genomes were based on 51 866 and 48 038 sequences, respectively.
Genome analysis
An initial set of open reading frames likely to encode proteins (coding sequences (CDSs)) were predicted as described previously (Heidelberg et al., 2004). All predicted proteins larger than 30 amino acids were searched against a non-redundant protein database (Heidelberg et al., 2004). Frameshifts and point mutations were detected and corrected where appropriate. The remaining frameshifts and point mutations were considered to be authentic. Protein membrane-spanning domains were identified by TopPred (Claros and von Heijne, 1994). Each CDS was inspected to define the initiation codon, the position of the ribosomal binding site and the transcription termination site. Two sets of hidden Markov models were used to determine CDS membership in families and superfamilies: Pfam (Bateman et al., 2004) and TIGRFAMs (Haft et al., 2003). Pfam hidden Markov models were also used with a constraint of a minimum of two hits to find repeated domains within proteins and to mask them. Phylogenomic analysis was used to assist with functional predictions, and comparative genome analyses were performed using the Comprehensive Microbial Resource (Peterson et al., 2001).
Comparative genome analysis
Putative orthologs of the Synechococcus OS-A and OS-B genomes were identified by reciprocal best-match BLAST comparisons. Those CDSs that did not fit this criterion were identified as being isolate-specific (Supplementary Table S3).
Metagenomic analyses
Metagenomic sequences were generated from high and low temperature samples of the microbial mats of Octopus and Mushroom Springs. The Synechococcus metagenomic sequences were classified into Synechococcus ‘OS-A-like’ or ‘OS-B′-like’ based on BLASTN analysis of the end reads against the complete genome sequences of Synechococcus OS-A and OS-B′. Classification into the OS-A or OS-B′-like bins required meeting the following criteria: (a) both ends of the clone insert had the best BLASTN score to the same genome (either to Synechococcus OS-A or OS-B′); (b) matches of both end sequences had a nucleotide identity >92% over at least 300 bp; (c) the distance between end-paired reads, based on their known genomic positions, could not be >25% of the average clone insert size; and (d) the paired reads had to come from opposite strands of the DNA (Supplementary Table S6). These sequences represent ∼17% of total metagenomic reads. By assembling the clones onto the anchor genomes, large metagenome scaffolds were created that spanned almost the entire genomes of Synechococcus OS-A and OS-B′ (86% with an average gap size of 931 bp and 89% with an average gap size of 617 bp for the Synechococcus OS-A and OS-B′ genomes, respectively). It is important to note that the genomic reconstruction resulting from this ‘stringent’ assembly is derived from sequenced genomic fragments from individual cells, and therefore represents a ‘virtual genome’, rather than the entire genome from an individual Synechococcus cell. The assemblies generated were annotated in the same way as for the completed genomes.
In the process of building assemblies from metagenomic sequences, we identified numerous clones with at least one end that matched the Synechococcus OS-A or OS-B′ anchor genomes, but that did not fulfill at least one of the four criteria described above. We refer to these as ‘illegal clones’. The inserts in the illegal clones (a) had a match to an anchor genome at one end of the clone, but not at the other end (this feature might represent a gene deletion or insertion, or a region that has undergone extensive sequence divergence); (b) had a match to an anchor genome at both ends, but the distance between the paired end reads was greater than expected (this feature might represent a rearrangement of the genome); (c) had a match to an anchor genome at both ends, but the sequences were both from the same strand (this feature might represent a transversion and recombination event); or (d) had a match to an anchor genome at both ends, but the match on one of the ends only covered a very short part of the read.
Genes ‘missing’ in the metagenome sequence
The region encoding urease subunits and accessory proteins (ureEFG), present in the Synechococcus OS-A genome appeared to be absent in the metagenome (see below, Figure 2). Clones that would be predicted to contain the urease accessory protein region were identified and sequenced to completion by transposon mutagenesis and transposon sequencing. The completely sequenced clone inserts were annotated as described above.
Transcript analysis and irradiance measurements
The level of the feoB gene transcript was monitored by quantitative PCR (qPCR) over the diel cycle using mat samples from Mushroom Spring (60°C site) (Steunou et al., 2006). The primers used for qPCR were feoB-F (5′-CGGGTTTGGTGATGAAAAGC) and feoB-R (5′-CCCACCGAATTTAACAAGCC). Irradiance measurements and the method for qPCR have been described previously (Steunou et al., 2006).
Results and discussion
Genome sequences of two Synechococcus isolates
The genomes of Synechococcus OS-A (2.9 Mbp) and OS-B′ (3.0 Mbp) have a relatively high G+C% content of 60.3 and 58.5 and include 2892 and 2933 predicted CDSs, respectively (Supplementary Table S1). There was no evidence of plasmids or phage-like genes on the chromosome of either of the Synechococcus isolates. Both genomes have two rRNA operons that are identical within each isolate (Figure 1). The 16S rRNA and 16S–23S rRNA internal transcribed spacer (ITS) sequences are identical to sequences previously characterized from mat samples, confirming that we had sequenced isolates from Synechococcus populations that are dominant in the mat (Papke et al., 2003). The Synechococcus OS-A and OS-B′ 16S and 23S rRNA sequences are 96.4% and 96.3% identical to each other, respectively, suggestive of significant divergence between the isolates, and yet the genomes of these isolates share a large fraction (∼83% based on bidirectional best BLAST scores) of their CDSs, and the CDSs exhibit a high identity between putative orthologs (∼87% amino-acid identity, ∼92% amino-acid similarity; ∼86% nucleotide identity, on average). A comparison of the Synechococcus OS-A and OS-B′ genomes revealed a marked lack of conserved, large-scale gene order, indicating an extensive history of rearrangement events (Figure 1). Regions of colinearity between the Synechococcus OS-A and OS-B′ genomes are short (∼70% of either genome is composed of conserved blocks of 1–2 kbp in length containing one or two genes), with the largest region of conserved gene order between the two isolates being ∼32 kbp and containing the genes involved in nitrogen fixation (Delcher et al., 2002; Steunou et al., 2006). In contrast, a comparison of the complete genomes of closely related bacteria usually reveals extensive conservation of large-scale genome architecture or synteny; even genomes that are not so closely related can show significant synteny (Rocap et al., 2003; Bentley and Parkhill, 2004). The lack of congruence between the measures of 16S rRNA identity, genome-wide identity between putative homologs, and genomic synteny of the two Synechococcus isolates implies that any one of these criteria by itself may not accurately reflect the level of relatedness between the Synechococcus isolates (Konstantinidis and Tiedje, 2005; Ward et al., 2006).
Genome rearrangements and recombination events are often mediated by transposons or phage (Bennett, 2004). Both Synechococcus OS-A and OS-B′ genomes contain many transposon-like or insertion sequence (IS) elements (109 and 98, respectively), but several of these are presumed non-functional as evidenced by truncations or putative frameshift mutations. The IS elements are not always located at the borders of rearranged regions, so their role in the large-scale gene re-rearrangements cannot be easily assigned (Parkhill et al., 2003). However, Synechococcus OS-B′ does contain 17 identical copies of an IS4 family of transposase genes (ISSoc13 or Interpro ID 002559), which are absent in the Synechococcus OS-A genome and which may still be active within the Synechococcus OS-B′-like organisms (Figure 1, circle 7, purple bars). Furthermore, both the Synechococcus OS-A and OS-B′ genomes contain a high frequency of an octameric, palindromic repeat (GGGATCCC), but the functional significance of this repeat is unclear. The presence of an internal GATC sequence within the repeat raises the possibility that they may be part of a DNA modification system that has been implicated in a number of processes ranging from restriction modification to DNA repair and transcriptional regulation (Wion and Casadesus, 2006) (Supplementary Table S2).
As expected from previous studies, both Synechococcus OS-A and OS-B′ contain genes encoding proteins required for photosynthesis, the biosynthesis of glycolate (Bateson and Ward, 1988), glycogen (Konopka, 1992; Nold and Ward, 1996), sulfolipids (Ward et al., 1994), and fermentative and respiratory metabolisms (Nold and Ward, 1996). We also identified genes required for the biosynthesis of Type IV pili and photoreceptors associated with phototaxis, which fits with earlier reports of motility of Synechococcus cells in the mats (Ramsing et al., 1997; Bhaya, 2004). However, the presence and activity of a functional pathway for nitrogen fixation (based on in situ expression nif genes and measurements of nitrogenase activity) in Synechococcus OS-A and OS-B′ was unexpected, as previous attempts had failed to measure nitrogen fixation in the mats (Steunou et al., 2006).
Identification of genes specific to Synechococcus OS-A or OS-B′
To identify functional differences between Synechococcus OS-A and OS-B′, we examined subsets of genes unique to each of these isolates. There are 393 and 503 isolate-specific CDSs in Synechococcus OS-A and OS-B′, respectively, but approximately half of these CDSs are annotated as either ‘hypothetical’ (172 and 218 in Synechococcus OS-A and OS-B′, respectively) or ‘conserved hypothetical’ (50 and 46 in Synechococcus OS-A and OS-B′, respectively), with other CDSs potentially encoding transposases/resolvases (91 and 89 in Synechococcus OS-A and OS-B′, respectively) (Supplementary Table S3). However, we were able to identify examples of genes encoding proteins with known functions that are present on only one of the genomes. For instance, only the Synechococcus OS-B′ genome harbors an 8 kbp region containing 10 phn-like genes (CYB_0159 to CYB_0168), which might enable the organism to transport (phnCDE) and metabolize (phnGHIJKLM) phosphonates. This may allow Synechococcus OS-B′ to utilized phosphonates as a source of phosphorus in addition to phosphate, the prevalent source of phosphorus in most environments. The region flanking the phn cluster is syntenic between the Synechococcus OS-A and OS-B′ genomes, indicating that the phn gene cluster was either recently acquired by Synechococcus OS-B′ or lost in Synechococcus OS-A (Figure 1). There is evidence suggesting that operons required for phosphonate uptake and utilization may be acquired through lateral gene transfer events in prokaryotes (Huang et al., 2005). Recently, genes for phosphonate utilization have been identified in metagenomic studies of marine, oxygenic photosynthetic prokaryotes, but the phn operon is not universally found in cyanobacteria, perhaps reflecting the different availability of phosphonates in various environments (Palenik et al., 2003; Dyhrman et al., 2006). A search for phn-like genes within the metagenome sequences identified 92 sequences that covered this region with high identity (that is, >92% NAID). Almost all originated from the recombinant libraries generated from Octopus or Mushroom Spring low-temperature regions of the mat, which is consistent with the observation that Synechococcus OS-B′-like organisms are more prominent in the lower temperature regions (Supplementary Table S4). There may be species unrelated to Synechococcus that can utilize phosphonate in the mats because there are other phn-like genes in the metagenome dataset that have low identity (∼55% AAID) to the phn genes of Synechococcus OS-B′. The origins, levels and importance of this and other phosphorus sources in the hot springs are currently being investigated.
Other genes present on the Synechococcus OS-B′ but not the Synechococcus OS-A genome are those encoding cyanophycin synthetase (CYB_0911) and cyanophycinase (CYB_2043). Cyanophycin is a nitrogen-rich reserve polymer synthesized non-ribosomally from aspartate and arginine by the enzyme cyanophycin synthetase; the polymer is degraded by cyanophycinase (Simon, 1987). Cyanophycin levels vary with growth conditions, but can be high in stationary-phase cultures or under conditions in which the growth potential of the cell decreases because of a limitation for nutrients such as sulfate or phosphate (Stevens and Poane, 1981). Cyanophycin has also been implicated in the integration of carbon and nitrogen metabolism in unicellular and filamentous cyanobacteria (Mackerras et al., 1990). The presence of cyanophycin synthetase and cyanophycinase on the Synechococcus OS-B′ genome suggests that this organism experiences fluctuating nitrogen levels; conditions of excess nitrogen may trigger cyanophycin storage, whereas periods of nitrogen limitation may result in cyanophycin degradation. Further experimental evidence in which gene expression in Synechococcus OS-B′ is measured under various nutrient regimes under defined laboratory conditions or in situ over the diel cycle, will allow us to address these questions.
Evidence of recent acquisition or loss of nutrient utilization pathways
We noted differences between the Synechococcus OS-A and OS-B′ isolates for genes required for the utilization of urea. Synechococcus OS-A has one genomic region encoding urease (ureA1B1C) and accessory factors (ureEFG1D1) (cluster 1 urease in Figure 2, top left), which is not present in Synechococcus OS-B′. Additionally, there are other regions in both isolates with remnants of genes encoding a second urease that is likely to be non-functional (Figure 2, bottom left). The genes of cluster 1 urease are flanked by transposons. The regions bordering the urease cluster (CYA_0598 and CYB_0030; CYA_0609 and CYB_0031; CYA_0610 and CYB_0033) are syntenic between Synechococcus OS-A and OS-B′, suggestive of a relatively recent gain of genes by Synechococcus OS-A, or loss of genes from Synechococcus OS-B′. The second set of urease-like genes in Synechococcus OS-A (ureA2, ureB2, and ureG2, ureD2, making up cluster 2A and 2B, respectively) are at two different genomic locations. The gene ureB2 (CYA_2585) is truncated by the integration of a transposon, whereas ureA2 (CYA_2588) and ureG2 (CYA_0751) contain frameshift mutations. A second ureC and ureF were not identified on the Synechococcus OS-A genome. In contrast, the Synechococcus OS-B′ genome contains a single copy of the ure genes that are located at five different regions of the genome. These genes have higher identity with the genes of Synechococcus OS-A cluster 2 than those of cluster 1, and in some cases regions flanking the cluster 2 urease genes in Synechococcus OS-A are syntenic with those flanking the homologous genes in Synechococcus OS-B′ (Figure 2, bottom left). In Synechococcus OS-B′ the cluster 2 urease genes have neither insertions nor frameshift mutations, and are therefore likely to represent functional genes. Also both Synechococcus OS-A and OS-B′ genomes contain genes encoding urea transport polypeptides (livFGMHK), which have very high identity between the isolates (∼99% amino-acid identity) (Figure 2, top right).
The functionality of the different urease genes has yet to be experimentally verified, but these obvious differences in gene content underscore the possibility that both gene gain and loss are ongoing events in the mat Synechococcus populations. The mechanisms underlying this genome fluidity and their evolutionary implications remain to be explored, but we speculate that a relatively recent acquisition of urease cluster 1 (flanked by transposons) by Synechococcus OS-A may have led to the progressive loss of functionality of the second urease cluster (still maintained by, and likely to be functional in Synechococcus OS-B′). We have recently developed an oligonucleotide microarray that will be used to query the isolate transcriptomes under different nutrient conditions, which will allow us to check the expression status of the urease gene clusters in Synechococcus OS-A and OS-B′.
Initial analysis of the metagenome sequence dataset indicated that sequences representing the ureEFG1D1 of the cluster 1 urease were absent (Figure 2, bottom right), raising the possibility that the Synechococcus OS-A anchor genome sequence may not be representative of the predominant Synechococcus OS-A-like populations in the mat. To clarify this, we identified and sequenced clones from the metagenome dataset that were predicted to span the region containing urease cluster 1 genes, based on clone-end read information. These clones (GYSA072 and YMBDB52) did contain the urease genes, so the apparent absence of these sequences in the metagenome dataset is possibly a reflection of a region that did not get sequenced at the same frequency as flanking regions. Thus, correlating sequence frequency data from metagenomic datasets with actual frequencies of genes in populations may require close attention to methodological constraints and statistical analysis of the data, followed by further verification before strong conclusions can be drawn about underrepresented genes in a metagenome database (Tringe et al., 2005).
Identification of functional diversity in the metagenome
The variations in nutrient acquisition and utilization capabilities suggested by differences in genome content between the two sequenced Synechococcus isolates raise the possibility that a detailed examination of Synechococcus-like sequences in the metagenome dataset might provide further examples of functionally specialized populations. To accomplish this, we characterized metagenomic sequences derived from both Mushroom and Octopus Springs at two different temperatures (Materials and methods and Supplementary Table S5), on the basis of identity to the Synechococcus anchor genomes. We found a significantly higher degree of identity of Synechococcus OS-A-like sequences in the metagenomic samples with the anchor genome (85% of the sequences with a best BLASTN score to the OS-A genome were within 2% divergence of the Synechococcus OS-A anchor genome) compared to that of the Synechococcus OS-B′-like sequences (only 50% of the sequences with a best BLASTN score to the Synechococcus OS-B′ genome were within 2% divergence of the Synechococcus OS-B′ anchor genome) (Figure 3). These results correlate well with the finding that there is a greater depth of rRNA divergence within the Synechococcus OS-B′-like population than within the Synechococcus OS-A-like population, and that there is generally less sequence variation among members of the Synechococcus OS-A-like population (Ward et al., 1998). The greater sequence diversity in the Synechococcus OS-B′-like than in the Synechococcus OS-A-like metagenome is also consistent with a greater diversity of ecotypes among the Synechococcus OS-B′-like organisms (Ward et al., 2006), as based on a simulation of ecotype evolution (Cohan and Perry, 2007).
Furthermore, identification of metagenomic sequences based on their source (for example, Octopus or Mushroom Springs, low or high temperatures) yielded a picture supporting the notion that temperature and spring characteristics represent important factors in shaping community diversity (Figure 3 and Supplementary Table S5). In accord with this idea, few Synechococcus OS-B′-like sequences were found in libraries from the higher temperature regions of Octopus or Mushroom Spring mats, whereas Synechococcus OS-A-like sequences were present in all four of the libraries, but represented a higher proportion of sequences in the those libraries constructed with DNA derived from mat samples from the higher temperature regions (Figure 3, and inset Table). These findings raise a number of interesting questions regarding the range of sequence variation within the Synechococcus OS-A and OS-B′ populations, which can be addressed by further analysis of the metagenomic sequence dataset or by using a targeted approach to examine particular genes or regions of interest.
Using stringent assembly criteria (see Materials and methods and Supplementary Table S6), 12 450 and 17 521 metagenome reads were assembled into scaffolds that were anchored to the Synechococcus OS-A and OS-B′ genome, respectively. These reads covered 86 and 89% of the Synechococcus OS-A and OS-B′ anchor genomes, respectively. 21 674 reads matched either the Synechococcus OS-A or OS-B′ genome, but the clones from which the read was derived could not be assembled onto the anchor genome because they failed to meet one of the assembly criteria (‘illegal clones’), and we surmised that they might represent regions in which recombination, transversion or gene gain or loss may have occurred. Hence, these clones represent a potentially rich source for analysis of genetic variation (Materials and methods and Supplementary Table S6).
We investigated a category of illegal clones in which one end of the clone had high sequence identity (>95% NAID) to a specific region on the Synechococcus OS-B′ genome, whereas the paired end sequence did not match any sequences in the Synechococcus OS-B′ genome. These clones could represent a Synechococcus population closely related to Synechococcus OS-B′ which contains additional sequences that are absent in the anchor genome. We identified several individual metagenome clones in which only one end of the clone matched the Synechococcus OS-B′ genomic region with high identity in the neighborhood of ∼0.565–0.577 Mb on the genome. To resolve how these ‘illegal’ clones differed from the anchor genome, we identified and sequenced a 7.6 kbp clone that matched the Synechococcus OS-B′ genome at both ends but contained an extra 5.5 kbp region relative to the Synechococcus OS-B′ anchor genome. In the Synechococcus OS-B′ genome, this region contains four genes, CYB_0562, CYB_0563, CYB_0564 and CYB_0565 (Figure 4, top). The metagenomic clone insert, however, contains seven additional CDSs, and is flanked by CYB_0562 (99.72% NAID) on the left and CYB_0565 (99.76% NAID) on the right (Figure 4a), whereas CYB_0563, CYB_0564 genes are absent. Of the genes present in the 5.5 kbp region two exhibited significant identity to the feoA (46% AAID to tlr1739) and feoB (64% AAID to tlr1740) genes of the unicellular thermophilic cyanobacterium, Thermosynechococcus elongatus.
The presence of the feoA and feoB genes in a Synechococcus OS-B′-like population is interesting because these genes are present in several bacteria where they encode proteins required for ferrous ion transport (Andrews et al., 2003). Iron is present in the environment as both ferrous and ferric forms, but the ferrous form predominates under conditions of low oxygen and is relatively soluble. Neither the Synechococcus OS-A nor OS-B′ anchor genomes contain feoA or feoB-like sequences, although they have several genes that function in ferric ion uptake and assimilation. The presence of feo genes in an organism that may be closely related to Synechococcus OS-B′ is interesting because it suggests the presence of functionally specialized populations with differential specificity for the different forms of iron. The functionality of the feo genes in the mat is supported by in situ analysis of feoB transcript levels (quantified using gene-specific primers for qPCR), which appear to peak in the afternoon, about 2 h before darkness; transcript levels stay low during the night and remain low as the cells are exposed to light in the morning (Figure 4, bottom). Thus, there may be an accumulation of the ferrous transport system as the mat becomes anoxic during the night, allowing some Synechococcus OS-B′-like organisms to scavenge the reduced ferrous ions that should become more plentiful as oxygen levels decrease in the mat.
These results provide an example of a comparison of metagenomic sequences with fully sequenced anchor genomes that has helped identify specialized functional populations that potentially have a different physiological capability and ecology. It is worth noting that so far, we have analyzed metagenomic clones that are relatively small (between 2 and 15 kbp), so we cannot easily place them into larger scaffolds with a high degree of certainty. Consequently, we are unable to decipher the degree of similarity between the organism from which this clone was derived and the Synechococcus OS-B′ anchor genome. However, screening of BAC libraries that contain much larger clones (>100 kbp) will allow us to identify large contiguous regions of genomes that contain these sequences. This will allow us to assess how similar these metagenomic clones are to the sequenced Synechococcus anchor genomes. The hypothesis that these feo containing organisms correspond to ecotypes different from that represented by Synechococcus OS-B′ would be supported if the feo-containing organisms were found to be members of distinct sequence clusters for widely shared genes (for example, recA, rpoB and lepA) (Cohan and Perry, 2007). Further analyses of the other classes of illegal clones will also allow us to create a more detailed picture of the level and kinds of functional variation that exists within the Synechococcus populations.
In summary, we have generated two ‘anchor’ genome sequences from Synechococcus OS-A and OS-B′, which represent dominant high- and low-temperature adapted in situ mat populations, respectively. Comparison of these two genomes revealed a striking lack of conserved large-scale genome architecture, suggestive of extensive genome rearrangements. Many obvious differences between these genomes appear to be related to the assimilation and storage of different nutrients such as nitrogen, phosphorus and iron. Further, population genetics and in situ distribution and expression analyses coupled with detailed physicochemical measurements will be required to ascertain whether the differences in gene complement observed constitute niche-adaptation strategies in the hot springs. The implications of the observations makes it important to define nutrient gradients and fluxes within the microbial mat communities, and to elucidate the ways in which these gradients impact the evolution of microbes in this environment.
We also analyzed metagenome sequences from the microbial mat community and compared them to the Synechococcus OS-A and OS-B′ anchor genomes. The spatial distribution and degree of diversity of the metagenomic variation is consistent with that for Synechococcus OS-A-like and OS-B′-like populations previously observed by using 16S rRNA and ITS sequences (Ward et al., 1998, 2006). Through comparative genomic analyses we have demonstrated that the genomes of these Synechococcus OS-A and OS-B′ isolates are not representative of all native Synechococcus OS-A and OS-B′ populations inhabiting the mat community that were sampled in our metagenomic sequences. Our analyses have revealed examples of functionally specialized populations that may have been derived from gene exchange and may define previously unknown Synechococcus OS-A-like or B′-like functional populations (that is, ecotypes). More extensive analysis of these genomic and metagenomic databases may reveal whether or not genomic fluidity is a more general phenomenon associated with hot spring mat communities, where organisms exist in close proximity and where DNA transfer through processes such as natural transformation or phage infections might occur with some frequency. To adequately address the question of niche adaptation, we will need to correlate functional differences (based on gene content and enzyme activity in situ) with ecological differences (based on microgeographic distribution) and sequence clustering of shared genes. As appreciation of, and information about, the astounding genetic diversity of microbes increases; it is also becoming obvious that population genetics, systematics, genomics and metabolic potential must be integrated to resolve complex issues about microbial communities.
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Acknowledgements
The research was funded by the Frontiers in Integrative Biology (FIBR) program at NSF (Grant EF-0328698). Natalia Khuri acknowledges a NSF-ROA Grant. The sequence of the chromosome of Synechococcus OS-A and Synechococcus OS-B′ have been deposited at GenBank (CP000239 and CP000240). Sequences of clones covering the feo region (EU189023); the urease region (EU189024 and EU189025) and metagenome sequences (Project IDs 20717, 20719, 20721,20723, 20725 and 20727) are also available at Genbank. Updates and further details on this project will be maintained at the following web sites: http://landresources.montana.edu/FIBR/ and http://fumarole.stanford.edu. We thank the Yellowstone National Park authorities for their excellent support. We also acknowledge the discussions with members of the Annual FIBR workshops held at the University of Montana, Bozeman.
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Bhaya, D., Grossman, A., Steunou, AS. et al. Population level functional diversity in a microbial community revealed by comparative genomic and metagenomic analyses. ISME J 1, 703–713 (2007). https://doi.org/10.1038/ismej.2007.46
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DOI: https://doi.org/10.1038/ismej.2007.46
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