Abstract
Microbial biotransformations have a major impact on contamination by toxic elements, which threatens public health in developing and industrial countries. Finding a means of preserving natural environments—including ground and surface waters—from arsenic constitutes a major challenge facing modern society. Although this metalloid is ubiquitous on Earth, thus far no bacterium thriving in arsenic-contaminated environments has been fully characterized. In-depth exploration of the genome of the β-proteobacterium Herminiimonas arsenicoxydans with regard to physiology, genetics, and proteomics, revealed that it possesses heretofore unsuspected mechanisms for coping with arsenic. Aside from multiple biochemical processes such as arsenic oxidation, reduction, and efflux, H. arsenicoxydans also exhibits positive chemotaxis and motility towards arsenic and metalloid scavenging by exopolysaccharides. These observations demonstrate the existence of a novel strategy to efficiently colonize arsenic-rich environments, which extends beyond oxidoreduction reactions. Such a microbial mechanism of detoxification, which is possibly exploitable for bioremediation applications of contaminated sites, may have played a crucial role in the occupation of ancient ecological niches on earth.
Author Summary
Microorganisms play a crucial role in nutrient biogeochemical cycles. Arsenic is found throughout the environment from both natural and anthropogenic sources. Its inorganic forms are highly toxic and impair the physiology of most higher organisms. Arsenic contamination of groundwater supplies is giving rise to increasingly severe human health problems in both developing and industrial countries. In the present work, we investigated the metabolism of this metalloid in Herminiimonas arsenicoxydans, a representative organism of a novel bacterial genus widespread in aquatic environments. Examination of the genome sequence and experimental evidence revealed that it is remarkably capable of coping with arsenic. Our observations support the existence of multiple strategies allowing arsenic-metabolizing microbes to efficiently colonize toxic environments. In particular, arsenic oxidation and scavenging may have played a crucial role in the development of early stages of life on Earth. Such mechanisms may one day be exploited as part of a potential bioremediation strategy in toxic environments.
Introduction
Although arsenic is most notorious as a poison threatening human health [1], recent studies suggest that arsenic species may have been involved in the ancestral taming of energy and played a crucial role in early stages in the development of life on Earth [2,3]. Further speculations involve this metalloid in the colonization of extraterrestrial environments containing high arsenic levels [4,5]. Presently, arsenic contamination of drinking water constitutes an important public health problem in numerous countries throughout the world [6]. Elevated concentrations typically derive from the weathering of arsenic-bearing minerals or from geothermal sources; lower amounts are of anthropogenic origin, e.g., smelting and mining industries.
Microorganisms are known to influence arsenic geochemistry by their metabolism, i.e., reduction, oxidation, and methylation [7,8], affecting both the speciation and the toxicity of this element. Arsenate (As[V]) is less toxic than arsenite (As[III]), but, paradoxically, resistance to As[V] requires its reduction to As[III], which will be extruded. On the other hand, arsenite oxidation, which was primarily thought to constitute a detoxification mechanism [9], may serve as an energy source in chemilithotrophic microorganisms [10]. Bacteria metabolizing toxic elements represent therefore an attractive tool to restore contaminated sites. In this respect, H. arsenicoxydans strain ULPAs1, which oxidizes As[III] into its less toxic and more easily immobilized form As[V], has been proposed for use in the first steps of arsenic bioremediation [11].
This heterotrophic microorganism, formerly called Caenibacter arsenoxydans ULPAs1, was isolated from the activated sludge of an industrial water treatment plant contaminated with heavy metals such as arsenic, lead, copper, and silver [12]. In the Burkholderiales order, its nearest phylogenetic relatives are members of the Oxalobacteraceae/Burkholderiaceae families, which contain several natural isolates with important biotechnological properties. For example, bacteria of the Paucimonas [13] and Collimonas [14] genera are known for their polyhydroxybutyrate depolymerase and chitinase activity, respectively. H. arsenicoxydans is a representative strain of a new genus comprising bacteria isolated from various aquatic environments, including contaminated, mineral and drinking water [12,15,16]. To gain further insight into the mechanisms that permit the microbial colonization of arsenic-rich environments, we investigated the physiology of H. arsenicoxydans by genetic and functional approaches. The results reported here, associated with descriptive and comparative genomics data, emphasize the metabolic versatility of this strain with regard to arsenic and the ability of microorganisms to restore liveable conditions within their ecological niche.
Results
General Genome Features
The H. arsenicoxydans genome consists of a single circular chromosome of 3,424,307 bp (Figure 1) with a total of 3,333 coding sequences (CDSs), among which 38% are of unknown function (Table 1). Surprisingly, any attempt to identify extrachromosomal elements in this strain by DNA sequencing, pulse-field electrophoresis, or plasmid purification was unsuccessful (unpublished data). This suggests that, unlike many microbes isolated from natural or anthropized environments, H. arsenicoxydans contains neither a second chromosome nor a (mega)plasmid. In bacteria, mobile genetic elements are known to play a major role in the acquisition of genes involved in adaptation to environmental stresses [17]. In line with this observation and in contrast to the situation in related microorganisms such as Ralstonia metallidurans [18], only a small number of complete or partial insertion sequences (IS) were identified in the genome of H. arsenicoxydans (Table S1). These IS elements represent 0.65% of the genome and belong to several families; i.e., IS3, IS30, and IS110. H. arsenicoxydans also contains more complex transposons or transposon remnants, but, unlike those identified in biomining strains used for metal recovery from gold-bearing arsenopyrite ores [19], they do not convincingly harbor arsenic-resistance determinants. Interestingly, all the complete ISs are inserted with their transposase genes in a clockwise orientation with respect to the orientation of the replication fork, suggesting some sort of interference between replication and IS stability.
Table 1.
The overall GC content of the H. arsenicoxydans genome is 54.3 % but seven regions exhibit a lower content and one region a higher content than the average (Figure 1). The presence of ISs was recorded in six of the low-GC modules. Remarkably, the region with the highest GC content (63%), harbors several CDSs (coding sequences) identified as homologs of phage and/or plasmid-like genes coding for proteins involved in chromosome partitioning, DNA topoisomerase, DNA helicase, and DNA recombination and repair (Table S2). This region, which covers ∼90 kb in the H. arsenicoxydans genome, is bordered by two tRNA genes at one end and one tRNA gene at the other end, and is flanked on one side by an integrase gene (Figure 2), suggesting a probable acquisition by an RNA-mediated horizontal gene transfer [20]. In terms of similarity, this island is clearly made of three main parts (Figure 2). The first one contains an arsenic-resistance cluster, also found in R. metallidurans, and, to a lesser extent, in Azoarcus sp. and Pseudomonas fluorescens. The second part of this region harbors a set of genes highly similar to part of the clc genomic island originally discovered in Pseudomonas sp. strain B13, which is known for its ability to degrade chloroaromatic compounds [21]. The clc element is almost 100% identical over the whole length (102 kb) to a chromosomal region in the chlorobiphenyl-degrading bacterium Burkolderia xenovorans LB400 [22]. Interestingly, a similar region of conserved synteny was observed in various proteobacteria such as R. metallidurans, P. fluorescens, Xanthomonas campestris, and Azoarcus sp., but none of the catabolic properties described in the clc element, mainly the clc and the amn operons (allowing 3-chlorobenzoate and 2-aminophenol degradation, respectively), were found in this part of the H. arsenicoxydans island (Table S2). Specific metabolic capabilities are found in the third part of this region, especially glutathione-dependent and -independent enzymatic activities involved in formaldelyde oxidation. Finally, several resistance genes found in the clc element of the compared genomes (e.g., mercuric resistance in R. metallidurans or ultraviolet-light resistance in P. fluorescens, Table S2) support a role for this genomic island in the adaptive response to stressful environmental conditions.
Carbon and Energy Metabolism
Many bacterial strains of the Burkholderiales order are able to flourish in diverse ecological niches and grow on various carbon sources. Surprisingly, H. arsenicoxydans can metabolize only a limited number of organic acids such as lactate, oxalate, succinate, and acetate; this is consistent with the presence of the corresponding functions on the chromosome and the absence of carbohydrate transporter genes such as those found in the phosphostranferase system (Table S3). In addition, the use of amino acids as a sole carbon and nitrogen source is supported by the ability of the strain to grow on tryptone and the presence in its genome of multiple operons coding for amino acid transport systems. In contrast, none of the pathways enabling carbon fixation from CO2 (i.e., genes coding for ribulose 1,5-biphosphate carboxylase/oxygenase and those involved in the Calvin cycle) are present or complete, in conformity with the chemoheterotroph metabolism of H. arsenicoxydans.
Genes involved in the biosynthesis or degradation of glycogen were not identified in the genome of H. arsenicoxydans. In contrast, the presence of the phbA-phbB gene cluster, which encodes a β-ketothiolase and an acetoacetyl-coenzyme A reductase, and phbC, coding for a poly-beta-hydroxybutyrate polymerase, is consistent with the accumulation in H. arsenicoxydans of poly-beta-hydroxybutyrate as an intracellular energy storage material (unpublished data), as recently demonstrated in Ralstonia eutropha [23]. Moreover, the genome contains all the genes encoding the inorganic phosphate transport and the phosphate-specific transport systems [24,25], as well as genes possibly involved in the synthesis of high-energy polyphosphate granules (Table S3), which may constitute an additional means of energy storage for H. arsenicoxydans.
The diversity of electron transfer mechanisms is of prime importance in the management of energy in ecosystems subjected to frequent fluctuations in their oxygen content, such as water treatment plants. Genomic data analyses suggest that H. arsenicoxydans can accommodate a wider range of oxygen concentrations than was initially anticipated [12,26]. Indeed, the H. arsenicoxydans genome harbors multiple respiratory pathways, permitting microorganisms to grow under aerobic, microaerobic, and anoxic conditions (Table S3). Reducing equivalents derived from organic compounds can enter energy-conserving electron transfer chains via a succinate dehydrogenase and three distinct formate dehydrogenases, none containing selenocysteine. Possible inorganic electron donors are reduced sulfur compounds (with the notable exceptions of sulphite and dimethyl sulphite) and As[III]. In contrast, no hydrogenase-encoding genes have been detected, suggesting that the strain may not gain energy from the oxidation of H2 to protons. At the oxidizing end of bioenergetic electron transfer chains, five terminal oxidases might be operative (Table S3). The two caa 3 cytochrome oxidases usually operate under high oxygen tension while bo 3, cbb 3, and bd oxidases are more specific to low-oxygen conditions [27]. All enzymes involved in anaerobic respiration via denitrification have been identified in the genome, i.e., nitrate, nitrite, nitrous oxide, and nitric oxide reductases. A β-proteobacterial cytochrome bc 1-complex serves as a coupling site in many of these energy-conserving chains [28].
The genome was explored to identify genes coding for cytochrome proteins possibly facilitating electron transfer between the Aox system and the bc1 complex and cbb3 cytochrome oxidase. The consensus sequence for the cytochrome c center is Cys-x-x-Cys-His, in which the histidine residue is one of the two axial ligands of the heme iron. Among the 56 putative heme-binding proteins we identified, Hear0476 was a particularly attractive candidate, because this protein was not predicted as a subunit of a cytochrome containing system, its coding gene was located immediately downstream of the aoxABC operon, and its expression was induced in the presence of arsenic (Table 2). This putative protein belongs to the c552 family and was named AoxD. Such a cytochrome has been shown to interact with the terminal cytochrome cbb3 in Helicobacter pylori [29], to play the role of electron carrier to the bc1 complex in ammonia-oxidizing bacteria [30], and to coprecipitate with As[III] oxidase protein in Alcaligenes faecalis [9]. We therefore propose that AoxD represents the electron transfer link between AoxAB proteins and the ccb3 cytochrome oxidase and bc1 complex in H. arsenicoxydans.
Table 2.
Finally, any attempt to cultivate H. arsenicoxydans ULPAs1 with As[III] as an electron donor source was unsuccessful; this organism requires an organic compound as an energy source. Moreover, neither selenate reductase nor respiratory arsenate reductase was identified in the genome. In Shewanella sp., this latter enzyme is encoded by the arrAB locus and allows anaerobic respiration with As[V] as a terminal electron acceptor [31].
Arsenic Stress and Metal Resistance
H. arsenicoxydans is not only resistant to arsenic but also to various heavy metals such as cadmium and zinc (Table S4). This observation is consistent with the presence in its genome of multiple metal-efflux operons (Figure S1), e.g., three cobalt-zinc-cadmium czc operons. However, except for arsenic, the resistance levels to toxic metals were much lower than those measured in the metallophilic R. metallidurans (Table S4), which contains multiple plasmid-encoded genes [18], suggesting a specific physiological adaptation of H. arsenicoxydans towards the arsenic.
Exposure to arsenic results in various biological effects, including DNA damage and oxidative stress [32,33]. H. arsenicoxydans exhibits both positive oxidase and catalase activities [12], in agreement with the presence of one catalase and two superoxide dismutase–encoding genes (Table 2). The genome also encodes at least one thioredoxin peroxidase, one peroxiredoxin, one thioredoxin reductase, and one hydroperoxide reductase. Moreover, genes coding for bacterioferritin and bacterioferritin comigratory protein, known to protect cells against toxic hydroxyl radicals resulting from iron overload, could also play a role in the adaptive response to oxidative stress [34]. In addition, the partial screening of a Tn5-lacZ mutant library demonstrated an induction of several genes involved in DNA recombination and repair, e.g., radA and polA, in the presence of arsenic (Table 2). Their inactivation in H. arsenicoxydans led to an important loss of viability following UV exposure, which was further decreased by arsenic (Figure S2). This suggests that the metalloid exerts a significant effect on DNA integrity.
Although arsenic methylation occurs widely in the environment, only a single bacterial methyltransferase (ArsM), has been characterized thus far [35]. Neither a homologous arsM gene nor arsenic methylation activity was detected in H. arsenicoxydans (unpublished data). In contrast, As[III] oxidation has been demonstrated in this organism [36], resulting from the expression of the aoxAB operon (Table 2). The AoxA-Rieske protein-encoding gene is located upstream from the AoxB catalytic subunit gene [36]. Examination of available sequencing data, including those from the Sargasso Sea metagenome [37], suggests a similar organization of putative As[III] oxidase genes in various microorganisms, e.g., Thermus thermophilus, Chloroflexus aurantiacus, and Aeropyrum pernix (Figure 3), but not in the facultative autotrophic arsenite-oxidizing bacterium Alkalilimnicola ehrlichei MLHE-1, in which no aox gene has been identified thus far [38]. However, comparison of the neighboring CDSs revealed a limited synteny of other genes belonging to the aoxAB cluster in most organisms, even though an “arsenic genes island” as defined in Alcaligenes faecalis [10] (i.e., aoxAB genes close to arsenate resistance genes [ars]), was found in H. arsenicoxydans and in other organisms such as Nitrobacter hamburgensis and Chlorobium phaeobacteroides. Remarkably, the second phosphate-specific transport locus identified in H. arsenicoxydans, which shows similarity with phosphate-specific transport systems in Serratia marcescens [39] and in Pseudomonas putida [40], is located in the vicinity of the aoxRSAB locus (Figure 3). This supports a link between arsenate, a structural analogue of phosphate, and phosphate transport. Finally, homologs of aoxRS, a two-component signal-transduction system identified in Agrobacterium tumefaciens [41], were found upstream from aoxAB in H. arsenicoxydans and most of the proteobacteria (Figure 3). Their inactivation by transposon mutagenesis led to a complete loss of arsenite oxidase activity (Figure S3). These genes were, however, not detected in the genome of other As[III]-oxidizing prokaryotes, which suggests important differences in aoxAB regulation among microorganisms.
Compared to most microorganisms, including R. metallidurans and the arsenic metabolizer Alkalilimnicola ehrlichei, which contain a single ars operon, H. arsenicoxydans is remarkable in that its genome harbors four different ars loci (Figure 1). Indeed, three clusters of genes involved in resistance to arsenic were identified from a DNA genomic library in complementation experiments with an E. coli strain in which the ars operon was deleted. They code for an ArsR regulator, an As[III] extrusion pump, an ArsH putative flavoprotein with no known function [42,43], and one or two arsenate reductases (ArsC), and confer a high level of resistance to arsenic (Figure 4). Moreover, in silico analysis of the genomic data revealed the presence in H. arsenicoxydans of a fourth operon that lacks the As[III] pump-encoding gene and cannot therefore confer resistance to arsenate. Its physiological raison d'être remains enigmatic. Quantitative analysis of the transporter-encoding gene mRNA demonstrated that the resistance operons are either constitutively expressed or induced in the presence of As[III] in H. arsenicoxydans (Figure S4; Table 2). These observations were further supported by differential proteomic analyses of the ArsH, ArsC, and ArsR proteins preferentially accumulated on bidimensional gels in the presence of arsenic (Figure S4;Table 2).
Four arsenate reductases (ArsCa) in these operons belong to the group typified by the Staphylococcus aureus enzyme [44]. The arsCa genes show a high sequence similarity and phylogenetic trees indicate that arsCa of loci 1, 2, and 4 arose from a recent gene duplication within the Herminiimonas lineage (Figure 5). The same is true for the ArsR regulator and ArsH-encoding genes (unpublished data). Loci 2 and 3 operons additionally harbor a second reductase gene, arsCb (Figure 4), which is homologous to that of the E. coli R773 plasmid [45]. An extensive analysis of available bacterial genome data shows that the simultaneous presence of arsCa and arsCb genes in arsenic resistance operons is common among α, β-, and γ-proteobacteria. The frequent occurence of both arsCs in one operon argues against a mere redundancy of functions but is rather in favour of specific roles for each enzyme. The S. aureus ArsC-type enzyme has been shown to use thioredoxin as a reductant [46] whereas the E. coli ArsC-type protein works with glutaredoxin [47]. It therefore seems likely that the association of ArsCa and ArsCb enzymes enables various metabolic pathways to contribute reducing equivalents to the arsenic detoxification reaction, further enhancing the efficiency of this process.
Finally, the membrane transporter proteins differ strongly between the first two loci and locus 3 (Figure 4). The latter contains an Acr3-type transporter [48], which is typical for α-, β-, and several γ-proteobacteria (Figure 5). The other loci both associate an ArsB-type transporter with ArsC reductases that cluster with homologous enzymes usually associated with the Acr3-type transporter. Moreover, ArsB-type efflux pumps seem to be the main rule in Firmicutes, ɛ-, and γ- proteobacteria (Figure 5). H. arsenicoxydans thus stands out among β-proteobacteria by its possession of two ArsB-type transporters in its ars operons.
Regulation and Colonization Functions
Natural isolates have to constantly monitor the physicochemical parameters of their environment, which explains why numerous regulator-encoding genes have usually been identified in their genomes. Except for histone-like nucleoid structuring protein (H-NS), a RNA/DNA-associated protein widespread in proteobacteria [49], the H. arsenicoxydans genome contains a complete set of genes coding for nucleoid-associated proteins such as HU, IHF, FIS, and Hfq. No gene coding for catabolite activator protein was identified, consistent with the lack of carbohydrate metabolism in H. arsenicoxydans. In contrast, the genome codes for the O2 responsive protein Fnr, enabling the modulation of the various respiratory pathways [50]. Moreover, 42 genes coding for histidine kinases and response regulators were identified, which correspond to more than 1% of the whole genome. They include those involved in the regulation of the resistance to or the detoxification of toxic metals and metalloids such as arsenic (Figure S3) and presumably copper (Figure S1). The genome also contains genes coding for a QseBC two-component regulatory system known to control flagellum synthesis and motility by quorum sensing. No gene leading to autoinducer synthesis was identified, but this does not rule out the existence of an unidentified quorum-sensing system.
Flagellar genes are mainly clustered at two loci in the chromosome and were shown to encode a polar flagellum (Figure S5 and Table 2). The rotation of this appendix is driven by sodium motive force, as demonstrated by the loss of motility of H. arsenicoxydans in the presence of 0.3 mM amiloride, an inhibitor of Na+/H+ antiporters (Figure S6). Surprisingly, the synteny in the first locus is highly reminiscent of that in E. coli, whose motility is known to depend on peritrichous flagella [51]. This region contains the flhDC master operon in H. arsenicoxydans, suggesting that the flagellum-encoding genes are organized in a mixed peritrichous/polar cascade in this organism. Such a novel hierarchical cascade most probably results from gene acquisition from multiple sources followed by DNA rearrangements.
Although the flagellum morphology was not affected by the presence of arsenic (Figure S5), at least with respect to length and width, an increased concentration of this toxic element resulted in a concomitant increase in bacterial motility on semisolid agar plates (Figure 6) and in flagellar gene expression (Table 2). Aside from iron, an element that is essential to life, no such effect occurred with other toxic elements tested, such as Co[II] (Figure 6), Cu[II], Sb[III], or As[V] (unpublished data). The hypothesis that arsenic contributes to the metabolism of H. arsenicoxydans was further supported by the positive chemotactic response shown by the strain towards As[III] (Figure 7A). This observation suggests that the bacterium is able to sense and respond to the presence of As[III] in the medium. The genome of H. arsenicoxydans contains 12 methyl-accepting chemotaxis proteins–encoding genes. As most of these genes have no predicted function, it is tempting to speculate that at least one of them plays a role in this mechanism.
To determine how arsenic contributes to motility, GFP strains were constructed and their swimming behaviour was studied using video microscopy methods. While the average swimming speed of H. arsenicoxydans was 30 μm/s, a 2-fold increase was observed in the presence of 2 mM As[III]. Disruption of aoxA or aoxB gene by a transposon insertion located at the 84th or the 335th codon, respectively, abolished the improvement in the swimming performances in the presence of As[III] but not in the presence of Fe[III] (Figure 6), which suggests that the strain may gain additional energy from the arsenic-oxidation process. The presence of aoxD, a cytochrome c552–encoding gene, in the vicinity of the aoxAB operon (Figure 3) further supports this hypothesis.
Finally, in contrast to related β-proteobacteria such as R. metallidurans, the genome of H. arsenicoxydans contains a type IV pilin gene cluster. This mannose-sensitive haemagglutinin-encoding gene may be of importance in the interaction between H. arsenicoxydans and the microflora present in its environment. Moreover, electron microscopy examination revealed the induction of a thick capsule when H. arsenicoxydans was cultivated in As[III]-containing medium (Figure S5). An operon of 18 genes present in the genome, induced in response to arsenic (Table 2) and possibly involved in the synthesis of exopolysaccharides (EPS), may play a role in this process. In addition, nanoparticles were shown to accumulate in the capsule of H. arsenicoxydans as compared to H. fonticola, a phylogenetically related strain that does not oxidize arsenic (Figure S7). Physicochemical analysis by transmission electron microscopy/energy dispersive X-Ray spectroscopy demonstrated the existence of a high arsenic content, suggesting for the first time a role for EPS in the scavenging of this toxic element (Figure 7B).
Discussion
Within the Oxalobacteraceae family, H. arsenicoxydans and the closely related strains H. aquatilis and H. fonticola represent a new genus comprising bacteria isolated from diverse aquatic environments. Microorganisms of this novel taxonomic group may therefore be widespread in such natural or anthropized ecosystems. The genome sequence and the physiology of H. arsenicoxydans further support the ability of this strain to grow in a wide range of environmental conditions, in particular with respect to oxygen concentrations. Moreover, genomic and experimental data demonstrated that this organism is capable of accommodating the presence of high concentrations of various toxic metals. More importantly, H. arsenicoxydans has evolved multiple processes not only to resist arsenic toxicity, such as DNA repair, oxidative stress resistance, and As[III] extrusion, but also to detoxify it for its own profit, such as As[III] oxidation and its probable involvement in energy metabolism. Some of these unusual genetic determinants, acquired most probably by horizontal gene transfer, are organized as genomic islands.
Remarkably, the versatile regulatory system of H. arsenicoxydans enables it to sense dynamic changes in arsenic concentration and to initiate motility and EPS synthesis for attachment to this metalloid. Such adaptive mechanisms may play a key role in the environment, allowing microorganims to efficiently flourish and colonize arsenic-rich ecosystems. Moreover, recent results suggest that microbial biofilms are involved in the adsorption and immobilization of metals such as Pb[II] [52] and Cr[III] [53]. These properties have been used in biorehabilitation of aqueous solutions contaminated with heavy metals [54]. The ability of H. arsenicoxydans to scavenge arsenic in an EPS matrix may be of prime importance in the context of bioremediation of contaminated environments, leading to the sequestration of this toxic metalloid.
To our knowledge, the genome of H. arsenicoxydans is the first to be fully characterized for an arsenic-metabolizing microorganism. The results presented here provide evidence that the ability of microbes to colonize arsenic-rich environments extends beyond the biotransformation of this toxic element. Although biochemical processes play an important role in arsenic release into the environment [7,8], the physiology of the microbes inhabiting extreme ecological niches may not be restricted solely to oxidoreduction reactions. In this respect, the positive chemotaxic response to the presence of arsenic and the scavenging of this element, associated with the transformation of As[III] into its less toxic form As[V], may have been key mechanisms in the colonization of the ancient environment on earth, allowing for the development of other microorganisms. In the near future, sequencing data for other arsenic-metabolizing organisms, combined with molecular biology, genetics, biochemistry, and biophysics approaches, will lead us to identify new arsenic-dependent processes. H. arsenicoxydans may therefore constitute a reference bacterium for further research towards a comprehensive analysis of the molecular mechanisms governing biological arsenic responses.
Materials and Methods
Genome sequencing, assembly, and annotation.
The complete genome sequence of H. arsenicoxydans was determined using the whole-genome shotgun method. Three genomic libraries were constructed, i.e., two plasmid libraries (obtained after mechanical shearing of DNA and cloning of generated 3–4 kb and 8–10 kb fragments into plasmids pcDNA2.1 (Invitrogen, http://www.invitrogen.com) and pCNS (a pSU18-derivative), respectively, and one BAC library to order contigs (obtained by partial digestion with Sau3A of the genomic DNA and the introduction of ∼20-kb fragments into pBeloBac11 (New England Biolabs, http://www.neb.com). From these libraries, 26,112, 7,680 and 3,840 clones, respectively, were end-sequenced using dye-terminator chemistry on ABI3730 sequencers (Applied Biosytems, http://www.appliedbiosystems.com). The Phred/Phrap/Consed software package (http://www.phrap.com) was used for sequence assembly and quality assessment [55–57]. About 732 additional reactions were necessary to complete the genomic sequence.
Using the AMIGene software (Annotation of MIcrobial Genes) [58], a total of 3,355 CDSs were predicted (and assigned a unique identifier prefixed with “HEAR”) and submitted to automatic functional annotation: BLAST searches against the UniProt database (http://www.uniprot.org) were performed to determine significant homology. Based on the biological representation of the translation process, we applied Bayesian statistics to create a score function for predicting translation start sites. We integrated together the ribosome binding site sequence, the distance between the translation start site and the ribosome binding site sequence, the base composition of the start codon, the nucleotide composition following start codons, and the expected distribution of proteins length. To further increase the prediction accuracy, we took into account the predicted operon structures. These elements were combined to create a score function and the highest score was selected for the translation start site predictions (Y. Makita, unpublished data). Protein motifs and domains were documented using the InterPro database (http://www.ebi.ac.uk/interpro). In parallel, genes coding for enzymes were classified using the PRIAM software [59]. TMHMM v. 2.0 was used to identify transmembrane domains [60], and SignalP 3.0 was used to predict signal peptide regions [61]. Finally, tRNAs were identified using tRNAscan-SE [62]. Sequence data for comparative analyses were obtained from the NCBI database (RefSeq section, http://www.ncbi.nlm.nih.gov/RefSeq). Putative orthologs and synteny groups (i.e., conservation of the chromosomal colocalisation between pairs of orthologous genes from different genomes) were computed between H. arsenicoxydans and all the other complete genomes as previously described [63]. Manual validation of the automatic annotation was performed using the MaGe (Magnifying Genomes, http://www.genoscope.cns.fr) interface, which allows graphic visualization of the H. arsenicoxydans annotations enhanced by a synchronized representation of synteny groups in other genomes. The H. arsenicoxydans nucleotide sequence and annotation data have been deposited in the EMBL database (http://www.ebi.ac.uk/embl; see accession numbers list below).
All these data (i.e., syntactic and functional annotations, and results of comparative analysis) were stored in a relational database, called ArsenoScope [63]. This database is publicly available via the MaGe interface at https://www.genoscope.cns.fr/agc/mage.
Genetic and molecular biology.
Mutations in genes induced by arsenic or mutant strains expressing GFP were obtained by random insertion of a mini-Tn5 and of a mini-Tn5 harboring a modified GFP-encoding gene [64], respectively. DNA manipulation and sequence analysis were performed as previously described [36]. These analyses showed that the KDM-7 gfp mutant strain used in the present study carries a mini-Tn5 insertion in hear1692, a CDS coding for a conserved hypothetical protein. RNA preparation, probe construction, and quantitative analysis of transcripts were performed as previously described [65].
The H. arsenicoxydans genomic library was constructed in plasmid pcDNA 2.1 (Invitrogen) as previously described [66]. About 60,000 clones were selected on LB plates supplemented with 100 μg/ml ampicillin and pooled. Large-scale plasmid DNA isolation was carried out using the JETstar kit (GenoMed, http://www.genomed.com). This library was used to transform the E. coli arsenic-susceptible strain AW3110. Clones of interest were selected on LB medium supplemented with 5mM AS[III].
Microbiological methods.
Strains were cultivated in a chemically defined medium (CDM) or in tryptone medium at 25 °C supplemented with 1.5% agar when required [12]. Minimal inhibitory concentrations and arsenite oxidase activity were determined on agar plates as previously described [36]. CDM supplemented with 1% tryptone and 0.3% agar was used to test bacterial motility as previously described [67]. Bacterial cell tracking was performed as follows: ULPAs1 strain was grown in CDM for 72 h and 0.5 ml of the cell culture was then transferred into 4.5 ml of fresh CDM medium containing 1% tryptone. Half of the cell culture was further incubated for 24h in the presence of 50ppm As[III], and the other half was incubated without As[III]. 30 min prior to the cell tracking procedure, 100ppm As[III] was added to the samples incubated with arsenic.
Bacterial survival after UV treatment was determined using a spot-plating technique [68]. Serially diluted cultures (10- to 109-fold) were spotted (5 μl) in triplicate onto CDM agar plates. Plates were then incubated for 72 h at 25 °C in the dark. Dilution with spots containing five to 30 colonies were counted, and the resulting average was expressed as the ratio of viable cells in treated cultures to those in untreated cultures. The wild-type strain H. arsenicoxydans and mutants strains polA::Tn5, recQ::Tn5, and radA::Tn5 were grown in CDM or CDM supplemented with 300ppm As[III]. Plates were irradiated for different lengths of time with UV light (254 nm) from a germicidal lamp at a rate of 5 J m−2 s−1 and then incubated in the dark as described above.
Chemotaxis assays were performed using a modified agarose plug method [69]. The sides of the chemotaxis chamber each consisted of two plastic strips 15 mm apart placed on a glass slide. A drop of molten low melting point agarose containing the substrate to be tested was placed on a coverslip that was reversed onto the plastic strips to form a chamber. Cells intended for chemotaxis assays were grown in the presence of arsenite As[III], collected, resuspended in chemotaxis buffer, and supplied with 0.5 mM acetate as an energy source before being flooded into the chamber.
Two-dimensional electrophoresis, mass spectrometry, and protein identification.
Isoelectric focusing was conducted using the horizontal Multiphor II system (Pharmacia) from 60 μg of protein loaded onto an 18 cm pH 4–7 immobilized pH gradient strip. To account for unspecific variations, eight gels—obtained by using two independent protein preparations extracted from four independent cultures—were run for each condition (in the presence or in the absence of arsenite). In-gel protein digestion of the spots was performed with an automated protein digestion system, MassPREP Station (Waters, http://www.waters.com), and the resulting peptide extracts were then directly analysed by nanoLC-MS/MS on an Agilent 1100Series capillary LC system (Agilent Technologies, http://www.home.agilent.com) coupled to a HCT Plus ion trap (Bruker Daltonics, http://www.bdal.com/) as previously described [65].
Protein identifications were performed directly in the uninterpreted genome database. The complete genome sequence of H. arsenicoxydans was fragmented in regular length segments of 7,500 bases with 2,000 overlapping bases, translated in the six possible reading frames, and imported into a local Mascot (Matrix Science, http://www.matrixscience.com) proteomic search engine. The matching peptides thus allowed the identification of the coding region directly on the genome sequence. These matching peptides were then exported to the MS-BLAST program [70] to identify the function of the proteins by homology with proteins of organisms that are present in the databases. Aside from the identification of proteins differentially regulated in the presence of arsenic, a large proteome map was generated. These proteomic results were compared to the computational genome annotation results, which allowed the correction of several translation start codons, therefore constituting an additional validation tool for computational predictions.
Steps of the interpretation were automated and compiled thanks to homemade software and the interactive proteomic map of H. arsenicoxydans is publicly available via the InPact interface at http://inpact.u-strasbg.fr.
Electron and fluorescence microscopy.
Bacterial cells were grown in CDM medium and stained with 0.1% (v/v) osmium tetroxide prepared in water as previously described [12].
H. arsenicoxydans gfp cells were tracked as follows: 600 μl of each cell suspension was poured into a well and the cells were excited with UV light for 200 ms. The image acquisition was performed with a Nikon 2000 Eclipse epifluorescence microscope (http://www.nikonusa.com) equipped with a CCD camera and gray scale 16-bit images were recorded. The frame of the images was 100 μm in size. The digitized fluorescent signals emitted by GFP-positive cells were taken every 243 ms during 25-s time periods. These sequences of images were further analyzed in the form of stacks using the image analysis software package ImageJ (http://rsb.info.nih.gov/ij). The swimming speed was measured in the absence or the presence of sublethal arsenic concentration as follows: all pictures in each dynamic image sequence (stack) were normalized by subtracting the background and the resulting image was run through a sharpening edges filter. The signal was then enhanced and a crosshair (mark and count) tool was used to manually mark each displacement of a given cell through the stack. A manual threshold was applied to remove any remaining background noise and all the stacks were transformed into 8-bit binarized images. The distance traveled by a cell between two positions (from one image to another) was calculated using a 2-D coordinate system. The (x, y) coordinates of the bacterial cells were evaluated and the distance traveled was calculated according to the following equation:
where y 1 and y 2 are the positions of the marked pixels (cell) on the y axis and x 1 and x 2, those on the x axis in two adjacent images. The time taken by the bacteria to perform this movement was calculated as the number of images containing the bacterium (traced frames) divided by the frame capture interval of four pictures per second, i.e., t = 4 * N traces. All the displacements of each tracked cell were then combined and the average speed of each cell in μm/s was calculated using the velocity formula . The final cost function giving the average velocity of a single cell was:
Three separate cell cultures, each in triplicate samples, were assayed. For each sample, three stacks of images were analyzed.
Physicochemical analysis of the nanoparticles contained in the capsule of H. arsenicoxydans were performed using transmission electron microscope/energy dispersive X-ray spectroscopy). In order to provide such observations, bacteria were grown in enriched arsenic medium for 48 hours. A 6 μl drop of 20-fold diluted suspension was put onto a C-coated copper microgrid and air-dried. The transmission electron microscope used is a Philips STEM 420 (http://www.research.philips.com) operated at 120 kV. Qualitative and quantitative analyses were carried out using an INCA (Oxford Instruments, http://www.oxford-instruments.com) X-ray microanalyser. Analyses demonstrated that nanoparticles contain a high amount of arsenic.
Supporting Information
Accession Numbers
The EMBL (http://www.ebi.ac.uk/embl) accession number for the genome of H. arsenicoxydans is CU207211.
Sequence information corresponding to genes or proteins identified in other genomes and presented in Figures 2, 3, and 5, respectively, was obtained from the National Center for Biotechnology Information GenBank database (http://www.ncbi.nlm.nih.gov/entrez) under the following accession numbers:
Figure 2 accession numbers: Azoarcus sp. EbN1 (NC_006513), Burkholderia xenovorans LB400 (NC_007951), Pseudomonas fluorescens Pf-5 (NC_004129), Ralstonia metallidurans CH34 (NC_007973), and Xanthomonas campestris 85–10 (NC_007508).
Figure 3 accession numbers: Aeropyrum pernix (NC_000854), Agrobacterium tumefaciens (DQ151549), Alcaligenes faecalis (AY297781), Burkholderia multivorans (NZ_AAVB01000013), Chlorobium phaero-bacteroides (NZ_AAIC01000001), Chloroflexus aurantiacus (NZ_AAAH02000003), Environmental sample 1(AACY01058630), Environmental sample 2 (AACY01082423), Nitrobacter hamburgensis (NC_007960.1), Rhodoferax ferrireducens (NC_007908), Roseovarius sp217 (NZ_AAMV01000002.1), Sulfolobus tokodai (BA000023.2), Thermus thermophilus HB8 (NC_006462), and Xanthobacter autotrophicus (NZ_AAPC01000006).
Figure 5 accession numbers: Acidovorax sp. (YP_987260.1), Alcaligenes faecalis (AAS45115.1), Alkalilimnicola ehrlichei (YP_743542.1), Azoarcus sp. (YP_159866.1), Azotobacter vinelandii (ZP_00416369.1), Bradyrhizobium japonicum (NP_769726.1), Burkholderia mallei (YP_105320.1), Burkholderia multivorans (ZP_01573333.1), Burkholderia pseudomallei (ZP_01333850.1), Burkholderia vietnamiensis (ZP_00422769.1), Chlorobium phaeobacteroides (YP_910947.1), Comamonas sp. (ABI49647.1), Comamonas testosteroni (ZP_01519258.1), Corynebacterium efficiens (NP_737487.1), Corynebacterium efficiens (NP_738111.1), Delftia acidovorans (ZP_01580151.1), Methylobacillus flagellatus (YP_545602.1), Nitrobacter hamburgensis (YP_571847.1), Nitrobacter winogradskyi (YP_319723.1), Polaromonas naphthalenivorans (YP_982812.1), Pseudomonas aeruginosa (NP_250969.1), Pseudomonas putida (NP_744860.1), Pseudomonas syringae (YP_234590.1), Ralstonia metallidurans (YP_582486.1), Rhodoferax ferrireducens (YP_524897.1), Rhodopseudomonas palustris (NP_948893.1), Rhodospirillum rubrum (YP_426538.1),Roseovarius nubinhibens (ZP_00960539.1), Rubrivivax gelatinosus (ZP_00242261.1), Rubrivivax gelatinosus (ZP_00243884.1), Shewanella oneidensis (NP_716169.1), Shigella flexneri (AAP17870.1), Shigella flexneri (NP_838060.1), Wolinella succinogenes (NP_906976.1), Xanthobacter autotrophicus (ZP_01198809.1), and Xanthobacter autotrophicus (ZP_01199778.1)
Acknowledgments
We thank C. Sasakawa for fruitful comments and F. Elsass and the Laboratory of Analytical Electron Microscopy (Institut National de la Recherche Agronomique, Versailles, France) for technical assistance in transmission electron microscopy experiments.
Abbreviations
- CDM
chemically defined medium
- CDS
coding sequence
- EPS
exopolysaccharide
- IS
insertion sequences
- nb
number
Footnotes
Competing interests. The authors have declared that no competing interests exist.
A previous version of this article appeared as an Early Online Release on March 5, 2007 (doi:10.1371/journal.pgen.0030053.eor).
Author contributions. DM contributed to genome annotation and data analysis and to the writing of the manuscript, and performed genetic and molecular biology experiments. CM contributed to genome annotation and to the writing of the manuscript, and coordinated software development for genome analysis (MaGe). SK and SW contributed to genome annotation and data analysis, and to physiology experiments. VB, CD, SM, BS, and JW performed the sequencing and finishing of the genome. MB, ET, VB, EK, and PO contributed to genome annotation and data analysis. WN analyzed the data. SC, ZR, and DV contributed to the automatic and manual annotation, to the analysis of genome information and to MaGe development. FAP, CC, EL, ET, and AVD contributed to proteomic data analysis. MH contributed to genome annotation and proteomic data analysis, and to the development of InPact web interface. AL contributed to genome annotation. DL contributed to genome annotation and electron microscopy experiments. YM contributed to software development. MC, SD, PS, and BS contributed to genome data analysis. BC, DDS, and NP contributed to physiology, biochemistry or biophysics experiments. MCL initiated the experimental work on H. arsenicoxydans and contributed to genome annotation. AD contributed to genome annotation and data analysis and to the writing of the manuscript. PNB coordinated the project, contributed to the analysis of genome information, and wrote the manuscript.
Funding. DM was supported by a grant from the French Ministry of Education and Research and CC by a Bruker Daltonics company fellowhip. Financial support came from the Institut Pasteur, the Université Louis Pasteur (ULP), the Consortium National de Recherche en Génomique (CNRG), and the Centre National de la Recherche Scientifique (CNRS). Transmission electron microscopy analysis was performed at the platform of the IBMP-CNRS (Strasbourg) cofinanced by CNRS, Région Alsace, ULP, and the Association de la Recherche pour le Cancer (ARC). ISfinder is supported by the CNRS and has received some support from the ARC. This work was done in the frame of the Groupement de Recherche–Métabolisme de l'Arsenic chez les Procaryotes (GDR2909-CNRS) (http://gdr2909.u-strasbg.fr).
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