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Keywords
- Okinawa Trough
- Optimal Growth Temperature
- Shallow Marine Environment
- Ferredoxin Oxidoreductase
- Hyperthermophilic Archaea
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Among the hyperthermophilic archaea, representatives of order Thermococcales form the most numerous group to date. Members of this group are the most frequently isolated hyperthermophiles. They are heterotrophic and as such regarded as the major constituents of organic matter within marine hot water ecosystems (Canganella et al., 1997). They belong to the branch of Euryarchaeota that contains the methanogens, the genus Thermoplasma, and the extremely halophilic archaea. The Thermococcales order is actually represented by three genera: Pyrococcus (Fiala and Stetter, 1986), Thermococcus (Achenbach-Richter et al., 1988) and the newly described Paleococcus (Takai et al., 2000). Phylogenetic analysis based on 16 rDNA sequences indicates that the Paleococcus strains are members of an ancient lineage of Thermococcales that diverged prior to the formation of the genera Pyrococcus and Thermococcus (Takai et al., 2000). These three genera include at present 38 species: 2 belonging to the genus Paleococcus, 6 belonging to the genus Pyrococcus, and 30 to the genus Thermococcus. The optimal growth temperature is 95–100°C for members of the genus Pyrococcus and 80–90°C for those of the genus Thermococcus. Pyrococcus strains have been isolated only from marine hydrothermal vents, whereas species belonging to the genus Thermococcus have been isolated also from terrestrial fresh water (Ronimus et al., 1997), marine solfataric ecosystems, deep-sea hydrothermal vents (Stetter, 1996) and offshore oil wells (Takahata et al., 2001). Representatives of the order Thermococcales have coccoid cells with or without flagella; they are obligate anaerobic organotrophic thermophiles with a fermentative metabolism using peptides, polysaccharides, or other sugars as carbon sources. Elemental sulfur is either stimulatory or necessary for the growth of these microorganisms. Molecular hydrogen that is produced during fermentation reduces elemental sulfur to H2S (Schönheit and Schäfer, 1995). Most of Thermococcales are neutrophiles growing optimally at pH 6.0–7.0; only the two species Thermococcus alcaliphilus (Keller et al., 1995) and T. acidoaminovorans (Dirmeier et al., 1998) are able to grow optimally at pH 9.0.
Ecology
The Thermococcales are generally found in natural biotopes that are typical for thermophilic microoganisms. They were originally discovered in terrestrial and submarine hot vents and they were then found also in deep subsurface environments. For example, Thermococcus celer (Zillig et al., 1983), T. litoralis (Britton et al., 1995) and Pyrococcus sp. were discovered in an offshore oil production platform in the North Sea (Stetter, 1996), and T. litoralis (Neuner et al., 1990) was isolated from a continental oil well (Paris Basin, France). This fact probably indicates the indigenous origin of hyperthermophilic archaea in the deep subsurface biosphere. Another strain, T. sibiricus, was isolated from a high temperature oil reservoir in Western Siberia, a location far remote from both the ocean and volcanic areas. The sites where these microorganisms are found can appear to be unusual, but these microorganisms might have been deposited with the original sediment and survived over geologic time by metabolizing buried organic matter (Miroshnichenko et al., 1998; Miroshnichenko et al., 2001).
On the other hand, members of the genus Pyrococcus seem to be isolated from only marine environments and belong to a particular ecological niche (Morikawa et al., 1994). As a result of the hydrostatic pressure at deep-sea vents, geothermally heated seawater remains liquid at temperatures up to 400°C (Stetter, 1996; Duffaud et al., 1998). When the hot fluid that is enriched in polymetal sulfides and gasses is mixed with cold (2°C) seawater, minerals precipitate and form so-called “chimneys,” or “smokers” (Fiala and Stetter, 1986). The temperature of the hot fluid that is emitted from the chimney can even reach 300°C (Holden and Baross 1993; Kwak et al., 1995; Gonzalez et al., 1998; Cambon-Bonavita et al., 2003). Members of the genus Pyrococcus are common inhabitants of this ecologic environment together with other hyperthermophiles belonging to the genera of Pyrodictium, Pyrobaculum, Pyrolobus and Methanopyrus. The two strains Pyrococcus abyssi and Paleococcus horikoshii were isolated from deep-sea vents of the North Fiji Basins, South Pacific Ocean (Erauso et al., 1993), and Okinawa Trough, Japan (Gonzalez et al., 1998), respectively. Pyrococcus furiosus and Pyrococcus woesei have been discovered along the marine solfataras of the island Vulcano (Italy). The novel barophilic archaeon belonging to the genus Palaeoococcus was collected from a deep-sea hydrothermal vent chimney at the Myojin Knoll in the Ogasawara-Bonin-Arc, Japan (Takai et al., 2000).
Isolation
For the isolation of hyperthermophilic archaea, complex anaerobic media are usually used which are prepared according to the Hungate technique (Blamey et al., 1999). After taking samples with special syringes, they should be inoculated into serum vials (25–100 ml) or Hungate tubes (10 ml) containing media under an anaerobic atmosphere of CO2 or N2. The 1000 ml of medium should also contain 0.2–1% of elemental sulfur and 10–100 µl of resazurin (1 mg/ml) as a redox indicator. Before inoculation, the medium should be reduced with sodium sulfide (Na2S; 0.05%). The sample may be transported at ambient temperature and kept at 4°C. Most Thermococcales may survive for a long time at cold or ambient temperature. Using special equipment, the samples taken from the deep sea can be transferred to the laboratory under pressure, and enrichment cultures can be prepared under high pressure and temperature. Samples from the deep sea can be collected by employing a manned submersible. In many cases and to increase the cell concentration, marine samples have to be concentrated many fold using a sterilized cross-flow device equipped with a 50-kDa cut-off membrane. For the growth and isolation of marine Thermococcales, the medium MB (Bacto Marine Broth, Difco) can be used and contains, in general, the following components per liter: bactopeptone, 5 g; bactoyeast extract, 1 g; Fe(III) citrate, 0.1 g; NaCl, 19.45 g; MgCl2, 5.9 g; NaSO4, 3.24 g; CaCl2, 1.8 g; KCl, 0.55 g; Na2CO3, 0.16 g; KBr, 0.08 g; SrCl2, 34 mg; H3BO3, 22 mg; Na-silicate, 4 mg; NaF, 2.4 mg; (NH4)NO3, 1.6 mg; and Na2HPO4, 8 mg; the final pH is adjusted to 7.6–7.8. If the complete medium from Difco is used, 37.4 g must be added to 1 liter of water. It is important to filter the medium using normal filter paper to prevent the possible precipitation of iron. The medium that is normally prepared for the cultivation of Pyrococcus species is as follows: KH2PO4, 0.5 g; NiCl2 · 6H2O, 2 mg; trace element solution (Balch et al., 1979), 10 ml; sulfur, 30 g; yeast extract, 1 g; peptone, 5 g; and resazurin, 1 mg. The pH has to be adjusted to 6.4–6.5. After boiling the above-mentioned media under N2 atmosphere, they should be cooled on ice and transferred under N2 atmosphere to 10-ml Hungate tubes and sterilized by autoclaving. Before use, the medium must be reduced with a sterile neutral solution of Na2S · 9H2O (0.5 g/liter).
To obtain single colonies on plates, the same media can be used including Gelrite (0.8%), and the plates should be stored in anaerobic jars under a N2 atmosphere at the desirable temperature.
Cultivation
Thermococcales are receiving increasing interest from academia and industry because they provide a unique source of stable biocatalysts and other products such as archaeal lipids and compatible solutes. However, until recently only low cell concentrations (107–108 cells/ml) could be obtained, making application studies very difficult. The main reason for this has to be ascribed to difficulties related to the production and purification of large quantities of biocatalysts and cell components. Special equipment is also needed to cultivate some strains under high pressure and temperature. Innovative bioreactor design to improve biomass yield is required. Because the accumulation of toxic compounds is thought to be responsible for low biomass yields, dialysis fermentation of Paleococcus woesei (Blamey et al., 1999) and P. furiosus has been performed for effective removal of low-molecular-mass components from the fermentation broth. Unlike many other heterotrophic hyperthermophiles, significant growth of P. furiosus is not dependent on the presence of elemental sulfur (S0). When dialysis membrane reactors were applied, a dramatic increase in cell yields was achieved (Krahe et al., 1996). The cultivation of the hyperthermophilic archaeon Pyrococcus furiosus (growth at 90°C) resulted in cell yields of 2.6 g · liter−1. For P. furiosus the optimum stirrer speed was 1,800 rpm, and neither hydrogen nor the metabolic products were found responsible for the comparatively low cell yield. The fermentation processes can be scaled-up from 3 liters to over 30 liters (up to 300 liters). The pilot plant scale offers the possibility of transferring the fermentation performance to a larger industrial scale. In recent experiments it was shown that even the results of the 1-liter dialysis reactor can be reproduced in 30-liter reactors using external dialysis modules. On the other hand, a method was described for growing P. furiosus in 600-liter fermentors (Verhagen et al., 2001), which resulted in the production of 500 g of cells (wet weight).
As already mentioned, Thermococcales, isolated from deep sea vents, are able to grow not only at high temperature but also at hydrostatic pressure around 20–30 MPa. Owing to practical difficulties, the growth and the metabolism of barophilic Thermococcales have been poorly investigated. It has been demonstrated that the upper growth temperature is extended at least 3°C when cells of P. abyssi are cultivated at 20 MPa. Similar higher thermotolerance and upward shift in the optimal temperature were observed also for P. endeavori at 22 MPa (Erauso et al., 1993). More detailed studies with Thermococcus peptonophilus (Canganella et al., 1997) and T. barophilus (Marteinsson et al., 1999) have also demonstrated that both species are barophilic. In fact, in both cases the growth rate at the optimal growth temperature was higher under in situ hydrostatic pressure than under lower pressure.
Identification and Morphology
In general, in phase contrast microscopy, all known species of Thermococcales appear as spherical cells, mostly as diploid forms constricted to various degrees owing to the duration of the division process throughout the whole generation time. When the cells of Thermococcales are compared to those of Sulfolobales and certain Thermoproteales, the Thermococcales cells are more round, slightly irregular, and their size varies from 0.5 to 2.5 µm. In the final stage of division of Thermoccoccales cells, the two daughter cells are connected by a thin string of cytoplasm enclosed by a membrane and S-layer. In general, cells show a Gram-negative reaction. Unlike all other strains, T. aggregans cells form chains, and cell aggregates are particularly characteristic of this strain. However, the formation of aggregates is not a general characteristic but occurs only after cultivation of the strain on yeast-tryptone extract (Canganella et al., 1998; Fig. 1a).
Electron microscopy of Thermococcales cells reveals the presence of monopolar polytrichous flagella in most of the species. For example, P. furiosus (Fiala and Stetter, 1986), P. woesei (Zillig et al., 1987), P. abyssi (Erauso et al., 1993), P. horikoshii (Gonzalez et al., 1998), T. acidoaminovorans (Dirmeier et al., 1998), T. peptonophilus (Gonzalez et al., 1995) and T. chitinophagus (Huber et al., 1996) are all characterized by the presence of a tuft of polar flagella. Nevertheless, this is not a rule. In other strains, the flagella have a fimbriate arrangement as observed for T. siculi (Grote et al., 1999; Fig. 1b). In the case of T. alcaliphilus (Keller et al., 1995), only a single flagellum is present and in the case of T. sibiricus, the flagella are completely absent (Miroshnichenko et al., 2001).
The cytoplasmic membrane (5–10 nm) of T. chitonophagus is covered by a bilayered cell envelope with an inner periplasmic space (15–20 nm) and an external, densely stained layer (5 nm), probably corresponding to a surface-layer protein (Huber et al., 1996). The described organization (structure) of the cytoplasmic membrane is more or less similar among the other members of Thermococcales. Thermococcales have the typical archaeal cytoplasmic membrane lipids (ether lipids), and some members also have simple diether lipids (mainly made up of one or two phospholipids) and trace amounts of tetraethers. The presence of two rare acyclic and cyclic glycerol diphytanyl tetraethers has been reported in T. chitinophagus (Huber et al., 1996). However, more detailed studies have been carried out on the lipid structure of T. hydrothermalis isolated from a deep-sea hydrothermal vent. On the basis of acid methanolysis and spectroscopic studies, the polar lipids (amounting to 4.5% [w/w] of the dry cells) included diphytanyl glycerol diethers and dibiphytanyldiglycerol tetraethers in a 45 : 55 ratio. No cyclopentane ring was present in the tetraethers. From the neutral lipids (0.4% [w/w] of the dry cells), four di- and tri-unsaturated acyclic tetraterpenoid hydrocarbons and low amounts of di- and tetraethers (occurring in free form) were identified. All are structurally related to lycopane. The presence of these hydrocarbons provides some evidence that lycopane, widely distributed in oceans, could be derived, at least partially, from the hydrocarbons synthesized by some hyperthermophilic archaea. Analysis of the uninoculated culture medium indicates that fatty acid derivatives and some steroid and triterpenoid compounds identified in the lipidic extract of the archaea probably originate from the culture medium (Lattuati et al., 1998).
Physiology and Metabolism
Most of Thermococcales species are obligate anaerobic organothrophic thermophiles that prefer to utilize polymeric substrates like proteins and carbohydrates (preferentially oligo- and polysaccharides) as carbon and energy sources. Elemental sulfur is required in some cases for the growth and is used as an electron acceptor to remove reducing equivalents that are produced during fermentation. However, these physiological characteristics are not the rule for all members of the order Thermococcales and some differences can be observed in the three genera Thermococcus, Pyrococcus and Paleococcus (Selig et al., 1997; Table 1).
Species of the genus Pyrococcus are heterotrophic and sulfur-reducing microorganisms. Growth is observed when complex organic substrates such as yeast extract, peptone, tryptone, meat extract, and peptides are used (Fiala and Stetter, 1986). Pyrococcus furiosusand P. woeseican also grow on various carbohydrates such as starch (Biller et al., 2002), glycogen, pullulan (Blumentals et al., 1990; Costantino et al., 1990), cellobiose and pyruvate (Kengen et al., 1993). Pyrococcus glycovorans grows on proteinaceous substrate and different carbohydrates and, in addition, it is able to use glucose as carbon source, a feature that appears to be unique in hyperthermophiles (Barbier et al., 1999). Pyrococcus abyssiand P. horikoshii are unable to grow on carbohydrates (Erauso et al., 1993; Gonzalez et al., 1998). Unlike the results reported in the literature, in many cases some members of Thermococcales can even grow on modified media in the absence of sulfur. Members belonging to the genus Thermococcus appear to grow mainly on media containing complex proteinaceous substrates such as yeast extract or tryptone as the sole carbon and energy source. Some species like Thermococcus peptonophilus, T. alcaliphilusand T. zilligiiare unable to grow on amino acid mixtures (Gonzalez et al., 1995; Keller et al., 1995). There are few reports on the successful cultivation of hyperthermophiles on defined minimal media. A minimal defined medium has been reported for the cultivation of Thermococcus acidoaminovorans, which uses defined amino acids as the sole energy source (Dirmeier et al., 1998). Thermococcus aggregansand T. aegaeicus strains instead are able to use carbohydrates as substrates. Thermococcus aggregans is able to grow on starch and maltose and T. aegaeicusalso utilizes starch but under a N2/CO2 atmosphere (Canganella, et al., 1998). Significant growth on maltose and slow growth on cellobiose were observed for T. hydrothermalis (Godfroy et al., 1997; Gruyer et al., 2002) and T. fumicolans (Godfroy et al., 1996). Interestingly, T. chitinophagus represents the only species able to grow on chitin as a carbon source (Huber et al., 1996). With the exception of T. stetteri(Miroshnichenko et al., 1989), T. profundus (Kobayashi et al., 1994; Kwak et al., 1995) and T. waiotapuoensis(Gonzalez et al., 1999), Thermococcus strains are stimulated by addition of sulfur, but sulfur is not absolutely required (Arab et al., 2000). The recently identified archaeon Palaeococcus sp. possesses most of the morphological and physiological properties typical of Thermococcales. It, however, displays an absolute requirement for either elemental sulfur or ferrous iron (Fe2+). The requirement for iron represents an ancient characteristic of early microbial metabolism, in light of geochemical data suggesting the properties of habitats occupied by microorganisms belonging to the order Thermococcales (Takai et al., 2000).
The generation time of the members of Thermococcales is the shortest among Archaea. The time range is between 25 min for T. peptonophilus and 70 min for T. stetteri. The doubling time of the strains belonging to the members of the genus Pyrococcusis around 30–35 min (Table 1).
Sugar and Peptide Degradation Pathways
As already described, many Thermococcales show heterotrophic growth on a variety of carbohydrates. This suggests that oligosaccharides with varying degrees of polymerization are transported into the cell and are subsequently hydrolyzed to glucose. Various studies have focused both on the transport of the saccharides into the cell and on the pathways that are used to degrade the glucose (Schönheit and Schäfer, 1995). For Thermococcus litoralis, a transport system for both maltose and trehalose has been described that probably represents an ATP-binding cassette (ABC) transporter (Horlacher et al., 1998; Xavier et al., 1999). The trehalose-maltose binding protein, TMBP, and the ATPase subunit, MalK, have been functionally expressed in Escherichia coli (Greller et al., 1999; Greller et al., 2001; Diederichs et al., 2000). These binding protein-dependent transport systems exhibit an unusually high affinity for the sugar, with a Km in the submicromolar range. While glycolysis in thermophilic bacteria proceeds in a conventional way, glucose catabolism by Thermococcales (as well as in other hyperthermophilic archaea) differs from the canonical pathways, involves novel enzymes, and shows unique control. In an effort to understand the metabolism of cellobiose in P. furiosus, a binding protein-dependent ABC transport system for oligosaccharides was discovered. The 70-kDa protein is responsible for the uptake of cellobiose and most other α-glucosides (Koning et al., 2001).
Two major pathways are known to be involved in the degradation of glucose in prokaryotes: the Embden-Meyerhof (EM) and the Entner-Doudoroff (ED) pathways. In general, they differ in the key enzyme acting on glucose or glucose-6-phosphate and in the subsequent aldolytic cleavage of the intermediates fructose-1,6 biphosphate (EM) and 2-keto-3-deoxy-6-phosphogluconate (ED). So far, sugar degradation has been analyzed in representative species of the genera Thermococcus and Pyrococcus. The analysis included 1) determination of 13C-labeling patterns by 1H- and 13C-NMR spectroscopy of fermentation products derived from pyruvate after fermentation of specifically 13C-labeled glucose by cell suspensions, 2) identification of intermediates of sugar degradation after conversion of 14C-labeled glucose by cell extracts, and 3) measurements of enzyme activities in cell extracts (Schönheit and Schäfer, 1995; De Vos et al., 1998). It has been established that in the three Thermococcales, P. furiosus, T. celerand T. litoralis, glycolysis appears to occur via a modified EM pathway. This pathway is unusual because the hexose kinase and phosphofructokinase steps are dependent on ADP rather than ATP, and a novel tungsten-containing enzyme termed “glyceraldehyde-3-phosphate:ferredoxin oxidoreductase” (GAPOR) replaces the expected glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and phosphoglycerate kinase. In contrast, other thermophilic Archaea (like Sulfolobus solfataricus and Thermoplasma acidophilum) degrade glucose via the ED pathway, and hyperthermophilic bacteria belonging to the order Thermotogales degrade glucose via conventional forms of the EM and ED pathways (Schönheit and Schäfer, 1995; De Vos et al., 1998). A final step in sugar fermentation is the conversion of acetyl-CoA into acetate that produces ATP. Also in this crucial step, the Thermococcales are unique because they have a single enzyme, an ADP-dependent acetyl-CoA synthase, while in bacteria this reaction is catalyzed by two different enzymes, phosphate acetyltransferase and acetate kinase (Fig. 2). In addition, P. furiosushas the capacity to convert pyruvate into alanine, which acts as an alternative electron sink. This reaction involves the combined activity of both alanine aminotransferase and glutamate dehydrogenase (Kengen et al., 1994).
The operation of a new glycolytic pathway was demonstrated in nongrowing cells of Thermococcus zilligii by isotopic enrichment analysis of the end products derived from fermentation of 13C-labeled glucose. The new pathway involves the formation of formate, derived from C-1 in glucose, via cleavage of a six-carbon carboxylic acid. The operation of a novel glycolytic strategy in T. zilligii with two branches diverging at the level of glucose-6-phosphate was demonstrated (Ronimus et al., 2001). Glucose is phosphorylated by an ADP-dependent hexokinase to glucose-6-phosphate, which is subsequently degraded by two glycolytic branches: an EM-type glycolytic pathway and a new route where formate is produced by a reaction involving cleavage of the C-1 carboxylic group of a six-carbon compound to yield formate and a pentose phosphate. By analogy with the pyruvate-formate-lyase reaction, it was suggested that the six-carbon compound is a β-ketoacid, such as 2-keto-3-deoxy-6-phosphogluconate, derived from 6-phosphogluconate. The contribution of the novel glycolytic branch was twice as high as that of the EM-type pathway when cells were grown on tryptone, and the inverse relationship was found for cells grown in the presence of glucose. This is the first report of a glycolytic pathway involving the formation of formate from C-1 in glucose. It is noteworthy that the most atypical member of the Thermococcales, T. zilligii, possesses also this unusual glycolytic feature (Ronimus et al., 1999; Ronimus et al., 2001).
The pathways of peptide metabolism have been well studied in P. furiosus. Amino acid catabolism in P. furiosusis thought to involve four distinct 2-keto acid oxidoreductases that convert transaminated amino acids into their corresponding coenzyme A (CoA) derivatives (Blamey and Adams, 1993; Mai and Adams, 1994; Mai and Adams, 1996; Heider et al., 1996). These CoA derivatives, together with acetyl-CoA produced from glycolysis via pyruvate, are then transformed to their corresponding organic acids by two acetyl-CoA synthetases unique to archaea, with concomitant substrate-level phosphorylation to form ATP. Alternatively, it has been postulated that depending on the redox balance of the cell, 2-keto acids are decarboxylated to aldehydes and then oxidized to form carboxylic acids by a second tungsten-containing enzyme, aldehyde:ferredoxin oxidoreductase (AOR; Mai and Adams, 1996). A third enzyme of this type, termed “formaldehyde:ferredoxin oxidoreductase” (FOR), is thought to be involved in the catabolism of basic amino acids (Roy et al., 1999; Adams et al., 2001).
Molecular Biology
The DNA G+C content of members of Thermococcales varies from 37.5 mol% for Pyrococcus woeseito 60 mol% for Thermococcus barossii. The abyssal strains P. abyssi, P. horiskoshii and P. glycovorans are characterized by a higher G+C (44–47 mol%) content than that of the coastal strains P. furiosus and P. woesei (38 mol%). A G+C content higher than 40 mol% is a typical feature of most Thermococcus species, but also in this genus, a distinction can be made. According to Godfroy et al. (1997), the strains of the genus Thermococcus can be divided on the basis of their G+C contents into the following two groups: 1) a group of strains with high G+C content (50–58 mol%), including the strains from shallow marine environment, T. celerand T. stetteri, and three deep-sea species T. profundus, T. peptinophilus and T. funiculans; and 2) a group of strains with low G+C content (38–47 mol%), including deep-sea strains of T. chitinophagus, T. alcaliphilus and T. barophilus, an organism from a shallow marine environment, T. litoralis, and the microorganism from a terrestrial high temperature oil reservoir, Thermococcus sibiricus (Table 1).
Phylogenetic studies based on 16S rDNA analysis reveal that Pyrococcus and Palaeococcus strains are clustered separately from Thermococcus species. However, the topology of the dendogram based on neighbor-joining algorithms clusters the Thermococcus species in a different number of branches, thus indicating that at the phylogenetic level, diversity in the same genus within high temperature environments is remarkable (Fig. 3).
The recent advances in genome projects have provided a considerable amount of data, which enables genomes of distant organisms to be compared in a comprehensive and integrative way. Comparisons of closely related species constitute a complementary approach crucial to the understanding of genome evolution. At the genomic level, these comparisons provide a unique opportunity to understand the mechanisms that determine chromosomal organization and evolution. At the proteomic level, this powerful strategy can be used to assess the genuine extent of gene losses and gains that lead to the observed divergence of coding capacity. Comparison of the genomes of Thermococcales has been already performed on three closely related species: Pyrococcus abyssi(Cohen et al., 2003; Genoscope website [{http:\\www.genoscope.cns.fr}]), Pyrococcus horikoshii (Kawarabayasi et al., 1998; Kawarabayasi et al., 2001; The National Institute of Technology and Evaluation(NITE) website [{http:\\www.bio.nite.go.jp}]) and Pyrococcus furiosus (Maeder et al., 1999; Lecompte et al., 2001; Environmental Genome Project sponsored by the National Institute of Environmental Health Sciences [{http:\\www.genome.utah.edu}]; ORNL website [{http:\\www.ornl.gov}{). Several genome features of P. abyssi, P. horikoshiiand P. furiosus affirm the close relationship among the three species, including similar G+C content and RNA elements, like rRNA and tRNA. At the genomic level, the comparison reveals that a differential conservation among four regions of the Pyrococcus chromosomes correlates with the location of genetic elements mediating DNA reorganization. At the proteomic level, the closer proximity of P. abyssi and P. horikoshii is affirmed by their average amino acid identity (77%) and their chromosomal organization. Nevertheless, the evolutionary distance between P. abyssiand P. horikoshii is not negligible relative to P. furiosusbecause the average amino acid identities are also high between P. furiosus and the two other species (72% with P. abyssiand 73% with P. horikoshii). The comparison of the three Pyrococcus species sheds light on specific selection pressure acting both on their coding capacities and on their evolutionary rates. The two independent methods, the “reciprocal best hits” approach and a new distance-ratio analysis, allow detection of the false orthology relationships within the Pyrococcus lineage. Such analyses reveal a high amount of differential gains and losses of genes since the three closely related species diverged. The resulting polymorphism is probably linked to an adaptation of these free-living organisms to differential environmental constraints.
Enzymology
Because members of Thermococcales grow at high temperature, their enzymes are highly thermoactive and thermostable. A large number of enzymes show no significant loss of activity after several hours at 100°C and are even active at temperatures that exceed the optimal growth temperature of the organism from which they were isolated (Bertoldo and Antranikian, 2002). These properties make hyperthermophiles very attractive for new biotechnological applications. To date, a large number of extracellular and intracellular enzymes have been characterized. They include the extracellular enzymes like amylases, pullulanases, α-glucosidases and proteases but also intracellular enzymes like dehydrogenases, oxidoreductases and DNA polymerases (Table 2). Interestingly, the ability of hyperthermophiles to produce cellulases, xylanases and pectinases seems to be very limited, and only in few cases the formation of cellobiohydrolase has been reported. Among the intracellular enzymes, the DNA polymerase and DNA ligase from Pyrococcus sp. (Southworth et al., 1996) and the DNA polymerase from Thermococcus strains especially have attracted further interest because of their potential in commercial applications to PCR. For reviews on the enzymology of hyperthermophilic archaea and their potential applications refer to the following articles (Sunna et al., 1997; Niehaus et al., 1999; Lévêque et al., 2000; Bertoldo and Antranikian, 2002; Bohlke et al., 2002).
Literature Cited
Achenbach-Richter, L., R. Gupta, W. Zillig, and C. R. Woese. 1988 Rooting the archaebacterial tree: The pivotal role of Thermococcus celer in archaebacterial evolution Syst. Appl. Microbiol. 10 231–240
Adams, M. W., J. F. Holden, A. L. Menon, G. J. Schut, A. M. Grunden, C. Hou, A. M. Hutchins, F. E. Jenney Jr., C. Kim, K. Ma, G. Pan, R. Roy, R. Sapra, S. V. Story, and M. F. Verhagen. 2001 Key role for sulfur in peptide metabolism and in regulation of three hydrogenases in the hyperthermophilic archaeon Pyrococcus furiosus J. Bacteriol. 183(2) 716–724
Arab, H., H. Volker, and M. Thomm. 2000 Thermococcus aegaeicus sp. nov. and Staphylothermus hellenicus sp. nov., two novel hyperthermophilic archaea isolated from geothermally heated vents off Palaeochori Bay, Milos, Greece Int. J. Syst. Evol. Microbiol. 50 Pt 6 2101–2108
Balch, W. E., G. E. Fox, L. J. Magrum, C. R. Woese, and R. S. Wolfe. 1979 Methanogens: Reevaluation of a unique biological group Microbiol. Rev. 43(2) 260–296
Barbier, G., A. Godfroy, J. R. Meunier, J. Querellou, M. A. Cambon, F. Lesongeur, P. A. Grimont, and G. Raguenes. 1999 Pyrococcus glycovorans sp. nov., a hyperthermophilic archaeon isolated from the East Pacific Rise Int. J. Syst. Bacteriol. 49 Pt 4 1829–1837
Bertoldo, C., and G. Antranikian. 2002 Starch-hydrolyzing enzymes from thermophilic archaea and bacteria Curr. Opin. Chem Biol. 2 151–160
Biller, K. F., I. Kato, and H. Markl. 2002 Effect of glucose, maltose, soluble starch, and CO2 on the growth of the hyperthermophilic archaeon Pyrococcus furiosus Extremophiles 6(2) 161–166
Blamey, J. M., and M. W. Adams. 1993 Purification and characterization of pyruvate ferredoxin oxidoreductase from the hyperthermophilic archaeon Pyrococcus furiosus Biochim. Biophys. Acta 1161(1) 19–27
Blamey, J., M. Chiong, C. Lopez, and E. Smith. 1999 Optimization of the growth conditions of the extremely thermophilic microorganisms Thermococcus celer and Pyrococcus woesei J. Microbiol. Meth. 38(1–2) 169–175
Blumentals, I. I., S. H. Brown, R. N. Schicho, A. K. Skaja, H. R. Costantino, and R. M. Kelly. 1990 The hyperthermophilic archaebacterium, Pyrococcus furiosus. Development of culturing protocols, perspectives on scaleup, and potential applications Ann. NY Acad. Sci. 589 301–314
Bohlke, K., F. M. Pisani, M. Rossi, and G. Antranikian. 2002 Archaeal DNA replication: Spotlight on a rapidly moving field Extremophiles 6(1) 1–14
Britton, K. L., P. J. Baker, K. M. Borges, P. C. Engel, A. Pasquo, D. W. Rice, F. T. Robb, R. Scandurra, T. J. Stillman, and K. S. Yip. 1995 Insights into thermal stability from a comparison of the glutamate dehydrogenases from Pyrococcus furiosus and Thermococcus litoralis Eur. J. Biochem. 229(3) 688–695
Cambon-Bonavita, M. A., F. Lesongeur, P. Pignet, N. Wery, C. Lambert, A. Godfroy, J. Querellou, and G. Barbier. 2003 Extremophiles, thermophily section, species description Thermococcus atlanticus sp. nov., a hyperthermophilic Archaeon isolated from a deep-sea hydrothermal vent in the Mid-Atlantic Ridge Extremophiles 7(2) 101–109
Canganella, F., J. M. Gonzalez, M. Yanagibayashi, C. Kato, and K. Horikoshi. 1997a Pressure and temperature effects on growth and viability of the hyperthermophilic archaeon Thermococcus peptonophilus Arch. Microbiol. 168(1) 1–7
Canganella, F., W. J. Jones, A. Gambacorta, and G. Antranikian. 1997b Biochemical and phylogenetic characterization of two novel deep-sea Thermococcus isolates with potentially biotechnological applications Arch. Microbiol. 167(4) 233–238
Canganella, F., W. J. Jones, A. Gambacorta, and G. Antranikian. 1998 Thermococcus guaymasensis sp. nov. and Thermococcus aggregans sp. nov., two novel thermophilic archaea isolated from the Guaymas Basin hydrothermal vent site Int. J. Syst. Bacteriol. 48 Pt 4 1181–1185
Cohen, G. N., V. Barbe, D. Flament, M. Galperin, R. Heilig, O. Lecompte, O. Poch, D. Prieur, J. Querellou, R. Ripp, J. C. Thierry, J. Van der Oost, J. Weissenbach, Y. Zivanovic, and P. Forterre. 2003 An integrated analysis of the genome of the hyperthermophilic archaeon Pyrococcus abyssi Molec. Microbiol. 47(6) 1495–1512
Costantino, H. R., S. H. Brown, and R. M. Kelly. 1990 Purification and characterization of an alpha-glucosidase from a hyperthermophilic archaebacterium, Pyrococcus furiosus, exhibiting a temperature optimum of 105 to 115 degrees C J. Bacteriol. 172(7) 3654–3660
De Vos, W. M., S. W. Kengen, W. G. Voorhorst, and J. Van der Oost. 1998 Sugar utilization and its control in hyperthermophiles Extremophiles 2 201–205
Diederichs, K., J. Diez, G. Greller, C. Muller, J. Breed, C. Schnell, C. Vonrhein, W. Boos, and W. Welte. 2000 Crystal structure of MalK, the ATPase subunit of the trehalose/maltose ABC transporter of the archaeon Thermococcus litoralis EMBO J. 19(22) 5951–5961
Dirmeier, R., M. Keller, D. Hafenbradl, F. J. Braun, R. Rachel, S. Burggraf, and K. O. Stetter. 1998 Thermococcus acidaminovorans sp. nov., a new hyperthermophilic alkalophilic archaeon growing on amino acids Extremophiles 2(2) 109–114
Duffaud, G. D., O. B. d’Hennezel, A. S. Peek, A. L. Reysenbach, and R. M. Kelly. 1998 Isolation and characterization of Thermococcus barossii, sp. nov., a hyperthermophilic archaeon isolated from a hydrothermal vent flange formation Syst. Appl. Microbiol. 21(1) 40–49
Erauso, G., Reysenbach, A. L., Godfroy, A., Meunier, J. R., Crump, B., Partensky, F., Baross, J. A., Marteinsson, V., Barbier, G., Pace, N. R., and Prieur, D. 1993 Pyrococcus abyssi sp. nov., a new hyperthermophilic archaeon isolated from a deep-sea hydrothermalvent Arch. Microbiol. 160 338–349
Fiala, G., and K. O. Stetter. 1986 Pyrococcus furiosus sp. nov. represents a novel genus of marine heterotrophic archaebacteria growing optimally at 100°C Arch. Microbiol. 145 56–61
Godfroy, A., J. R. Meunier, J. Guezennec, F. Lesongeur, G. Raguénès, A. Rimbault, and G. Barbier. 1996 Thermococcus fumicolans sp. nov., a new hyperthermophilic archaeon isolated from a deep-sea hydrothermal vent in the north Fiji Basin Int. J. Syst. Evol. Microbiol. 46(4) 1113–1119
Godfroy, A., F. Lesongeur, G. Raguenes, J. Querellou, E. Antoine, J. R. Meunier, J. Guezennec, and G. Barbier. 1997 Thermococcus hydrothermalis sp. nov., a new hyperthermophilic archaeon isolated from a deep-sea hydrothermal vent. Int J. Syst. Bacteriol. 47 622–626
Gonzalez, J. M., C. Kato, and K. Horikoshi. 1995 Thermococcus peptonophilus sp. nov., a fast-growing, extremely thermophilic archaebacterium isolated from deep-sea hydrothermal vents Arch. Microbiol. 164(3) 159–164
Gonzalez, J. M., Y. Masuchi, F. T. Robb, J. W. Ammerman, D. L. Maeder, M. Yanagibayashi, J. Tamaoka, and C. Kato. 1998 Pyrococcus horikoshii sp. nov., a hyperthermophilic archaeon isolated from a hydrothermal vent at the Okinawa Trough Extremophiles 2(2) 123–130
Gonzalez, J. M., D. Sheckells, M. Viebahn, D. Krupatkina, K. M. Borges, and F. T. Robb. 1999 Thermococcus waiotapuensis sp. nov., an extremely thermophilic archaeon isolated from a freshwater hot spring Arch. Microbiol. 172(2) 95–101
Greller, G., R. Horlacher, J. DiRuggiero, and W. Boos. 1999 Molecular and biochemical analysis of MalK, the ATP-hydrolyzing subunit of the trehalose/maltose transport system of the hyperthermophilic archaeon Thermococcus litoralis J. Biol. Chem. 274(29) 20259–20264
Greller, G., R. Riek, and W. Boos. 2001 Purification and characterization of the heterologously expressed trehalose/maltose ABC transporter complex of the hyperthermophilic archaeon Thermococcus litoralis Eur. J. Biochem. 268(14) 4011–4018
Grote, R., L. Li, J. Tamaoka, C. Kato, K. Horikoshi, and G. Antranikian. 1999 Thermococcus siculi sp. nov., a novel hyperthermophilic archaeon isolated from a deep-sea hydrothermal vent at the Mid-Okinawa Trough Extremophiles 3(1) 55–62
Gruyer, S., E. Legin, C. Bliard, S. Ball, and F. Duchiron. 2002 The endopolysaccharide metabolism of the hyperthermophilic archeon Thermococcus hydrothermalis: Polymer structure and biosynthesis Curr. Microbiol. 44(3) 206–211
Heider, J., X. Mai, and M. W. Adams. 1996 Characterization of 2-ketoisovalerate ferredoxin oxidoreductase, a new and reversible coenzyme A-dependent enzyme involved in peptide fermentation by hyperthermophilic archaea J. Bacteriol. 178(3) 780–787
Higgins, D. G., J. D. Thompson, and T. J. Gibson. 1996 Using CLUSTAL for multiple sequence alignments Meth. Enzymol. 266 383–402
Holden, J. F., and J. A. Baross. 1993 Enhanced thermotolerance and temperature-induced changes in protein composition in the hyperthermophilic archaeon ES4 J. Bacteriol. 175(10) 2839–2843
Horlacher, R., K. B. Xavier, H. Santos, J. DiRuggiero, M. Kossmann, and W. Boos. 1998 Archaeal binding protein-dependent ABC transporter: Molecular and biochemical analysis of the trehalose/maltose transport system of the hyperthermophilic archaeon Thermococcus litoralis J. Bacteriol. 180(3) 680–689
Huber, R., J. Stöhr, S. Hohenhaus, R. Rachel, S. Burggraf, H. W. Jannasch, and K. O. Stetter. 1996 Thermococcus chitonophagus sp. nov., a novel, chitin-degrading, hyperthermophilic archaeum from a deep-sea hydrothermal vent environment Arch. Microbiol. 64 255–264
Kawarabayasi, Y., M. Sawada, H. Horikawa, Y. Haikawa, Y. Hino, S. Yamamoto, M. Sekine, S. Baba, H. Kosugi, A. Hosoyama, Y. Nagai, M. Sakai, K. Ogura, R. Otsuka, H. Nakazawa, M. Takamiya, Y. Ohfuku, T. Funahashi, T. Tanaka, Y. Kudoh, J. Yamazaki, N. Kushida, A. Oguchi, K. Aoki, and H. Kikuchi. 1998 Complete sequence and gene organization of the genome of a hyper-thermophilic archaebacterium, Pyrococcus horikoshii OT3 DNA Res. 5(2) 55–76
Kawarabayasi, Y. 2001 Genome of Pyrococcus horikoshii OT3 Meth. Enzymol. 330 124–134
Keller, M., F. J. Braun, R. Dirmeier, D. Hafenbradl, S. Burggraf, R. Rachel, and K. O. Stetter. 1995 Thermococcus alcaliphilus sp. nov., a new hyperthermophilic archaeum growing on polysulfide at alkaline pH Arch. Microbiol. 164(6) 390–395
Kengen, S. W., E. J. Luesink, A. J. Stams, and A. J. Zehnder. 1993 Purification and characterization of an extremely thermostable beta-glucosidase from the hyperthermophilic archaeon Pyrococcus furiosus Eur. J. Biochem. 213(1) 305–312
Kengen, S. W., F. A. de Bok, N. D. van Loo, C. Dijkema, A. J. Stams, and W. M. de Vos. 1994 Evidence for the operation of a novel Embden-Meyerhof pathway that involves ADP-dependent kinases during sugar fermentation by Pyrococcus furiosus J. Biol. Chem. 269(26) 17537–17541
Kobayashi, T., Y. S. Kwak, T. Akiba, T. Kudo, and K. Horikoshi. 1994 Thermococccus profundus sp. nov., a new hyperthermophilic archaeon isolated from a deep-sea hydrothermal vent Syst. Appl. Microbiol. 17 232–236
Koning, S. M., M. G. Elferink, W. N. Konings, and A. J. Driessen. 2001 Cellobiose uptake in the hyperthermophilic archaeon Pyrococcus furiosus is mediated by an inducible, high-affinity ABC transporter J. Bacteriol. 183(17) 4979–4984
Krahe, M., G. Antranikian, and H. Märkl. 1996 Fermentation of extremophilic microorganisms FEMS Microbiol. Rev. 18 271–285
Kwak, Y. S., T. Kobayashi, T. Akiba, K. Horikoshi, and Y. B. Kim. 1995 A hyperthermophilic sulfur-reducing archaebacterium, Thermococcus sp. DT1331, isolated from a deep-sea hydrothermal vent Biosci. Biotechnol. Biochem. 59(9) 1666–1669
Lattuati, A., J. Guezennec, P. Metzger, and C. Largeau. 1998 Lipids of Thermococcus hydrothermalis, an archaea isolated from a deep-sea hydrothermal vent Lipids 33(3) 319–326
Lecompte, O., R. Ripp, V. Puzos-Barbe, S. Duprat, R. Heilig, J. Dietrich, J. C. Thierry, and O. Poch. 2001 Genome evolution at the genus level: Comparison of three complete genomes of hyperthermophilic archaea Genome Res. 11(6) 981–993
Lévêque, E., S. Janeek, and H. B. Belarbi. 2000 Thermophilic archaeal amylolytic enzymes Enz. Microb. Technol. 1 3–14
Maeder, D. L., R. B. Weiss, D. M. Dunn, J. L. Cherry, J. M. Gonzalez, J. DiRuggiero, and F. T. Robb. 1999 Divergence of the hyperthermophilic archaea Pyrococcus furiosus and P. horikoshii inferred from complete genomic sequences Genetics 152(4) 1299–1305
Mai, X., and M. W. Adams. 1994 Indolepyruvate ferredoxin oxidoreductase from the hyperthermophilic archaeon Pyrococcus furiosus. A new enzyme involved in peptide fermentation J. Biol. Chem. 269(24) 16726–16732
Mai, X., and M. W. Adams. 1996 Purification and characterization of two reversible and ADP-dependent acetyl coenzyme A synthetases from the hyperthermophilic archaeon Pyrococcus furiosus J. Bacteriol. 178(20) 5897–5903
Marteinsson, V. T., J. L. Birrien, A. L. Reysenbach, M. Vernet, D. Marie, A. Gambacorta, P. Messner, U. B. Sleytr, and D. Prieur. 1999 Thermococcus barophilus sp. nov., a new barophilic and hyperthermophilic archaeon isolated under high hydrostatic pressure from a deep-sea hydrothermal vent Int. J. Syst. Bacteriol. 49 Pt 2 351–359
Miroshnichenko, M. L., E. A. Bonch-Osmolovskaya, A. Neuner, N. A. Kostrikina, N. A. Chernych, and V. A. Alekseev. 1989 Thermococcus stetteri sp. nov., a new extremely thermophilic marine sulfur-metabolizing archaebacterium Syst. Appl. Microbiol. 12 257–262
Miroshnichenko, M. L., G. M. Gongadze, F. A. Rainey, A. S. Kostyukova, A. M. Lysenko, N. A. Chernyh, and E. A. Bonch-Osmolovskaya. 1998 Thermococcus gorgonarius sp. nov. and Thermococcus pacificus sp. nov.: Heterotrophic extremely thermophilic archaea from New Zealand submarine hot vents Int. J. Syst. Bacteriol. 48 Pt 1 23–29
Miroshnichenko, M. L., H. Hippe, E. Stackebrandt, N. A. Kostrikina, N. A. Chernyh, C. Jeanthon, T. N. Nazina, S. S. Belyaev, and E. A. Bonch-Osmolovskaya. 2001 Isolation and characterization of Thermococcus sibiricus sp. nov. from a Western Siberia high-temperature oil reservoir Extremophiles 5(2) 85–91
Morikawa, M., Y. Izawa, N. Rashid, T. Hoaki, and T. Imanaka. 1994 Purification and characterization of a thermostable thiol protease from a newly isolated hyperthermophilic Pyrococcus sp Appl. Environ. Microbiol. 60(12) 4559–4566
Neuner, A., H. W. Jannasch, S. Belkinn, and K. O. Stetter. 1990 Thermococcus litoralis sp. nov.: S new species of extremely thermophilic marine archaebacterium Arch. Microbiol. 153 205–207
Niehaus, F., C. Bertoldo, M. Kahler, and G. Antranikian. 1999 Extremophiles as a source of novel enzymes for industrial application Appl. Microbiol. Biotechnol. 51(6) 711–729
Ronimus, R. S., A. Reysenbach, D. R. Musgrave, and H. W. Morgan. 1997 The phylogenetic position of the Thermococcus isolate AN1 based on 16S rRNA gene sequence analysis: A proposal that AN1 represents a new species, Thermococcus zilligii sp. nov Arch. Microbiol. 168(3) 245–258
Ronimus, R. S., J. Koning, and H. W. Morgan. 1999 Purification and characterization of an ADP-dependent phosphofructokinase from Thermococcus zilligii Extremophiles 3(2) 121–129
Ronimus, R. S., E. de Heus, and H. W. Morgan. 2001 Sequencing, expression, characterisation and phylogeny of the ADP-dependent phosphofructokinase from the hyperthermophilic, euryarchaeal Thermococcus zilligii Biochim. Biophys. Acta 1517(3) 384–391
Roy, R., S. Mukund, G. J. Schut, D. M. Dunn, R. Weiss, and M. W. Adams. 1999 Purification and molecular characterization of the tungsten-containing formaldehyde ferredoxin oxidoreductase from the hyperthermophilic archaeon Pyrococcus furiosus: The third of a putative five-member tungstoenzyme family J. Bacteriol. 181(4) 1171–1180
Schönheit, P., and T. Schäfer. 1995 Metabolism of hyperthermophiles World J. Microbiol. Biotechnol. 11 26–57
Selig, M., K. B. Xavier, H. Santos, and P. Schonheit. 1997 Comparative analysis of Embden-Meyerhof and Entner-Doudoroff glycolytic pathways in hyperthermophilic archaea and the bacterium Thermotoga Arch. Microbiol. 167(4) 217–232
Southworth, M. W., H. Kong, R. B. Kucera, J. Ware, H. W. Jannasch, and P. F. B. 1996 Cloning of thermostable DNA polymerases from hyperthermophilic marine Archaea with emphasis on Thermococcus sp. 9°N-7 and mutations affecting 3’-5’ exonuclease activity PNAS 93 5281–5285
Stetter, K. O. 1996 Hyperthermophiles in the history of life CIBA Found. Symp. 202 1–10; discussion 11–8
Sunna, A., M. Moracci, M. Rossi, and G. Antranikian. 1997 Glycosyl hydrolases from hyperthermophiles Extremophiles 1(1) 2–13
Takahata, Y., T. Hoaki, and T. Maruyama. 2001 Starvation survivability of Thermococcus strains isolated from Japanese oil reservoirs Arch. Microbiol. 176(4) 264–270
Takai, K., A. Sugai, T. Itoh, and K. Horikoshi. 2000 Palaeococcus ferrophilus gen. nov., sp. nov., a barophilic, hyperthermophilic archaeon from a deep-sea hydrothermal vent chimney Int. J. Syst. Evol. Microbiol. 50 Pt 2 489–500
Verhagen, M. F., A. L. Menon, G. J. Schut, and M. W. Adams. 2001 Pyrococcus furiosus: Large-scale cultivation and enzyme purification Meth. Enzymol. 330 25–30
Xavier, K. B., R. Peist, M. Kossmann, W. Boos, and H. Santos. 1999 Maltose metabolism in the hyperthermophilic archaeon Thermococcus litoralis: Purification and characterization of key enzymes J. Bacteriol. 181(11) 3358–3367
Zillig, W., I. Holtz, D. Janecovic, W. Schäfer, and W. D. Reiter. 1983 The archaebacterium Thermococcus celer represents a novel genus within the thermophilic branch of the archaebacteria Syst. Appl. Microbiol. 4 88–94
Zillig, W., I. Holz, H. P. Klenk, J. Trent, S. Wunderl, D. Janekovic, E. Imsel, and B. Haas. 1987 Pyrococcus woesei, sp. nov., an ultra-thermophilic marine Archaebacterium, representing a novel order, Thermococcales Syst. Appl. Microbiol. 9 62–70
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Bertoldo, C., Antranikian, G. (2006). The Order Thermococcales. In: Dworkin, M., Falkow, S., Rosenberg, E., Schleifer, KH., Stackebrandt, E. (eds) The Prokaryotes. Springer, New York, NY. https://doi.org/10.1007/0-387-30743-5_5
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