Abstract
Thermus sp. strain CCB_US3_UF1 is a thermophilic bacterium of the genus Thermus, a member of the family Thermaceae. Members of the genus Thermus have been widely used as a biological model for structural biology studies and to understand the mechanism of microbial adaptation under thermal environments. Here, we present the complete genome sequence of Thermus sp. CCB_US3_UF1 isolated from a hot spring in Malaysia, which is the fifth member of the genus Thermus with a completely sequenced and publicly available genome (Genbank date of release: December 2, 2011). Thermus sp. CCB_US3_UF1 has the third largest genome within the genus. The complete genome comprises of a chromosome of 2.26 Mb and a plasmid of 19.7 kb. The genome contains 2279 protein-coding and 54 RNA genes. In addition, its genome revealed potential pathways for the synthesis of secondary metabolites (isoprenoid) and pigments (carotenoid).
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Introduction
Thermus spp. are Gram-negative, aerobic, non-sporulating, and rod-shaped thermophilic bacteria. Thermus aquaticus was the first bacterium of the genus Thermus that was discovered in several of the hot springs in Yellowstone National Park, United States [1]. A few years later, two strains of Thermus thermophilus (HB27 and HB8) were successfully isolated from thermal environments in Japan [2, 3]. To date, many strains of Thermus have been isolated from various geothermal environments such as hot springs and deep-sea hydrothermal vents. In addition to the ability to survive under thermal environments, T. thermophilus can also thrive in environments with extreme pH values, demonstrating great capabilities for adaptation to various environmental conditions.
The whole genome sequences of two strains of T. thermophilus , HB8 and HB27, were independently completed in 2004 [4, 5]. The genome of a second Thermus species, Thermus scotoductus SA-01, is also available [6]. T. thermophilus has attracted attention as one of the model organisms for structural biology studies because protein complexes from extremophiles are easier to crystallize than their mesophilic counterparts [7]. Some of the breakthrough examples of large complexes from thermophiles that have been crystallized are structures of the 70S ribosome [8], the bacterial RNA polymerase [9, 10] and the respiratory complex I [11] from Thermus spp. that were solved before those of Escherichia coli .
Members of the genus Thermus are of considerable biotechnological interest as sources of thermophilic enzymes [12, 13]. Thermozymes and proteins from the genus Thermus are good candidates for industrial processes because of their high thermal stability and co-solvent compatibility. The most well-known enzyme mined from the genus Thermus is DNA polymerase, an important enzyme used in PCR. Other than DNA polymerase, thermozymes from this genus are also widely used in food, pharmaceutical and paper-pulp industries [7]. Examples of industrial applications for thermostable enzymes include organic synthesis (e.g. esterases, lipases, proteases), starch-processing (e.g. α-amylases, glucose isomerases), pulp and paper manufacturing (e.g. xylanases) as well as animal feed and human food production (amino acid and vitamin synthesis) [13, 14]. Here, we present a summary of classification and a set of features for Thermus sp. CCB_US3_UF1, together with the description of the complete genome sequence and annotation.
Organism information
Classification and features
Thermus spp. are suggested to be closely related to the genus Deinococcus based on several comparative studies on 16S rRNA and protein sequences, and they form a distinct branch known as the Deinococcus-Thermus group [15, 16]. Nevertheless, the exact phylogenetic position of the Deinococcus-Thermus phylum remains to be determined. This phylum was proposed to derive from the oldest groups of the Bacteria Domain, after those of Aquifex and Thermotoga based on 16S rRNA sequence comparison [17]. A more in-depth analysis of the phylogeny of the Deinococcus-Thermus phylum based on conserved orthologs can be carried out as genome sequences from both of the genera are available [18].
In order to better understand the phylogeny of Thermus sp. CCB_US3_UF1, we constructed a phylogenetic tree based on the 16S rRNA gene sequences. There are two identical copies of the 16S rRNA gene in the Thermus sp. CCB_US3_UF1 genome. One copy of the gene sequence was used to search against the nucleotide database using NCBI BLASTN [19]. The BLASTN result shows that it has the highest sequence identity to Thermus igniterrae RF-4 (97 %, Y18406), Thermus brockianus YS38 (96 %, Z15062), and Thermus scotoductus Se-1 (95 %, AF032127). Figure 1 shows the phylogenetic neighborhood of Thermus sp. CCB_US3_UF1 relative to type strains of the families Deinococcaceae and Thermaceae . Chloroflexus aurantiacus (D38365) was used as an outgroup to root the tree.
Thermus sp. CCB_US3_UF1 is a Gram-negative bacterium (Table 1) and it has a rod-shaped filamentous structure (Fig. 2). Members of the genus Thermus are capable of growing at temperatures ranging between 45 °C and 83 °C [20]. Most of them have a maximum temperature for growth at slightly below 80 °C [21, 22]. Interestingly, a few strains of T. thermophilus can grow at 80 °C or above [23]. Thermus sp. CCB_US3_UF1 was isolated from a hot spring in Ulu Slim, Perak, Malaysia. It can grow well between 60 °C and 70 °C. Thermus spp. need carbohydrates, amino acids, carboxylic acids and peptides as sources of carbon and energy. The strain CCB_US3_UF1 is an aerobic, non-sporulating, non-motile and yellow-pigmented bacterium. Some of the members of the genus Thermus are capable of growing anaerobically using nitrate as an electron acceptor and some can even reduce nitrite [22, 23].
Genome sequencing and annotation
Genome project history
The genus Thermus belongs to one of the oldest evolutionary branches of the Bacteria domain. The genome sequencing of Thermus sp. CCB_US3_UF1 was initiated as it can serve as a model bacterium for studying the evolution of thermophilic adaptation. The sequencing and finishing of the genome were completed at the Advanced Studies in Genomics, Proteomics and Bioinformatics (University of Hawaii) and TEDA School of Biological Sciences and Biotechnology (Nankai University, China). The genome annotation was performed at the Centre for Chemical Biology (Universiti Sains Malaysia). This genome sequence was first published in March 2012 [24]. A summary of the project information is shown in Table 2.
Growth conditions and genomic DNA preparation
Thermus sp. CCB_US3_UF1 was grown aerobically to late exponential phase in 50 ml of ATCC medium 697 ( Thermus medium) [3] at 60 °C. Genomic DNA was isolated from Thermus sp. CCB_US3_UF1 using a modified phenol-chloroform extraction protocol [25]. The quality of DNA was checked by 0.5 % agarose gel electrophoresis and its quantity by a NanoDrop 2000 Spectrophotometer (Thermo Scientific, Wilmington, Delaware, USA). A DNA concentration of 363.4 ng/μl and OD260/OD280 of 1.90 was obtained.
Genome sequencing and assembly
The whole-genome sequencing of Thermus sp. CCB_US3_UF1 was performed using Roche 454 and Illumina paired-end sequencing technologies. A 3 kb genomic library was constructed and 97,991 paired-end reads and 54,397 single-end reads were generated using the GS FLX system, providing 21.14-fold genome coverage. Six large scaffolds including 51 contigs were successfully assembled from 97.09 % of the reads using the 454 Newbler assembly software (454 Life Sciences, Branford, CT). A total of 3,469,788 reads from 3 kb library were produced to reach a depth of 115-fold coverage with an Illumina GA IIx (Illumina, San Diego, CA). These reads were mapped to the scaffolds using the Burrows-Wheeler Alignment (BWA) tool [26]. The majority of the gaps within the scaffolds were filled by local assembly of 454 and Illumina reads. The gaps between the scaffolds were filled by sequencing PCR products using an ABI 3730xl capillary sequencer. PCR products were sequenced to verify repeats larger than 3 kb. The putative sequencing errors were verified and corrected by consensus of the Roche/454 and Illumina reads.
Genome annotation
The automated annotation of the genome was done using the DIYA (Do-It-Yourself Annotator) pipeline [27]. The pipeline uses Glimmer3 to predict open reading frames [28], followed by protein similarity searches using BLAST [19] against UNIREF [29], RPS-BLAST against CDD [30], and Asgard [31]. In addition, RPS-BLAST searches against the COG database was done to enable assignment of COG functional categories to the ORFs. Transfer RNAs were predicted by using tRNAscan-SE [32] while ribosomal RNAs were identified by using RNAmmer [33].
Genome properties
The complete genome of Thermus sp. CCB_US3_UF1 is composed of a single circular chromosome of 2,243,772 bp and a plasmid of 19,716 bp with G + C contents of 68.6 % and 65.6 %, respectively (Fig. 3). There are 2334 predicted coding sequences (CDS), 2 rRNA operons, and 48 tRNA genes in the chromosome (Table 3). A total of 32 CDS are predicted in the plasmid. The distribution of genes into COG functional categories is presented in Table 4.
Comparison with other sequenced genomes
The genome of Thermus sp. CCB_US3_UF1 (2.26 Mb) is larger than those of T. thermophilus HB27 (2.13 Mb) and T. thermophilus HB8 (2.12 Mb), but smaller than that of T. scotoductus SA-01 (2.36 Mb) (Table 5).
The Thermus sp. CCB_US3_UF1 genome was compared against closely related Thermus genomes using BLAST and Artemis comparison tool to identify regions of synteny. The three closest Thermus with sequenced genomes ( T. thermophilus strains HB27, HB8 and T. scotoductus SA-01) were selected for the comparison. The genome of strain HB27 consists of a chromosome (1.89 Mb) and a megaplasmid (0.23 Mb). On the other hand, strain HB8 has a chromosome of 1.85 Mb, a megaplasmid (0.26 Mb) and a plasmid (9.3 kb) [5]. The genome of T. scotoductus includes a 2.3 Mb chromosome and a plasmid of 8.4 kb.
Thermus sp. CCB_US3_UF1, T. thermophilus HB27, HB8 and T. scotoductus SA-01 all have a small genome size that is below 2.5 Mb. They also display a high G + C content that may correlate with their thermophilic lifestyle. CCB_US3_UF1 has a higher number of predicted protein coding sequences (2279) than HB27 (2210) and HB8 (2173), but lower than that of T. scotoductus SA-01 (2458). They also share a similar number of rRNA (16S-23S-5S) operons with a well-balanced high G + C content above 60 %, a common feature displayed by thermophilic bacteria. The number of tRNAs that are present in all four genomes is between 47 and 48. In terms of transposase genes, T. scotoductus SA-01 has the highest number (22 genes), followed by CCB_US3_UF1 (13 genes), T. thermophilus HB27 (18 genes), and HB8 (18 genes). Interestingly, no prophage-related genes are found in these four genomes, implying the occurrence of clustered regularly interspaced short palindromic repeats (CRISPRs). CRISPR is characterized as a type of antiviral immune system found in Bacteria and Archaea [34].
There are 1728 proteins, or 76 % of the total proteins, from Thermus sp. CCB_US3_UF1 that are found orthologous to the proteins in T. thermophilus HB27, and a total of 1691 (74 %) orthologs are shared between CCB_US3_UF1 and T. thermophilus HB8. Meanwhile, a total of 1885 (83 %) proteins are shared between CCB_US3_UF1 and T. scotoductus SA-01, showing greater similarity between these two species. The protein ortholog mapping was done with a cut-off e-value of 10-5 using the protein-protein BLAST (blastp). Despite of the similarity of many of their gene products, genome-wide synteny between Thermus sp. CCB_US3_UF1 and T. thermophilus HB27, HB8 and T. scotoductus SA-01 could not be detected.
The plasmid of Thermus sp. CCB_US3_UF1 shows no overall similarity to the other sequenced plasmids of T. thermophilus HB27 and HB8, but it has high similarity to the plasmid of Thermus sp. 4C, designated as pL4C [35]. The gene encoding chromosome segregation ATPase (TCCBUS3UF1_p160) that is found in pL4C is present in the Thermus sp. CCB_US3_UF1 plasmid. This protein has been suggested to play an essential role in plasmid replication and partition [36]. In addition, a putative integrase gene that facilitates gene transfer and chromosome modification can be found in both plasmids.
Insights from the genome sequence
The Thermus sp. CCB_US3_UF1 genome encodes genes for complete tricarboxylic cycle, gluconeogenesis, glyoxylate bypass and Embden-Meyerhof pathways. Both Thermus sp. CCB_US3_UF1 and T. thermophilus HB27 share similar sets of genes that are involved in aerobic respiration. At high temperatures, the solubility of oxygen in water is low. Two terminal cytochrome oxidases are found in Thermus : a caa3- type (TCCBUS3UF1_540-550) that is expressed under high oxygen levels, and a ba3- type oxidase (TCCBUS3UF1_13990, TCCBUS3UF1_14010) that is expressed under low oxygen supply [37, 38]. Thermus sp. CCB_US3_UF1 is able to synthesize many important compounds, including amino acids, vitamins, cofactors, carriers, purines and pyrimidines. Many of these biosynthetic pathways show a high degree of conservation between CCB_US3_UF1 and T. thermophilus HB27. In addition, Thermus sp. CCB_US3_UF1 has branched-chain amino acid ABC transport systems that are important for nutrient acquisition, and ion transporters for the elimination of toxic compounds such as copper and arsenite.
Motility and natural transformation
So far, motility is not observed in Thermus and no flagella biosynthetic gene is present in the genomes. However, genes encoding gliding motility proteins (TCCBUS3UF1_13970, TCCBUS3UF1_13980) and a twitching mobility protein (PilT, TCCBUS3UF1_9080) are found in the genome of Thermus sp. CCB_US3_UF1. These two proteins are also found in T. thermophilus HB27, HB8 and T. scotoductus SA-01, and this raises the question regarding the existence of motility in Thermus .
Thermus sp. CCB_US3_UF1 is also found to possess type IV pili that are crucial in the attachment, twitching motility, surface colonization, and natural transformation systems in bacteria [39]. The efficiency of a DNA uptake system in T. thermophilus is crucial to thermoadaptation and exchange of genetic materials in high temperature environments. Competence proteins play an important role in natural transformation and can be categorized into three groups: DNA-translocator-specific proteins, type IV pili (Tfp)-related proteins, and nonconserved proteins [40]. Genes encoding DNA-translocator-specific proteins [ComEA (TCCBUS3UF1_22560), ComEC (TCCBUS3UF1_22570), DprA (TCCBUS3UF1_18680)] and Tfp-related proteins [PilA1 (TCCBUS3UF1_8740), PilA2 (TCCBUS3UF1_8720), PilA3 (TCCBUS3UF1_8710)] were found in the Thermus sp. CCB_US3_UF1 genome. Genes encoding leader peptidase (PilD, TCCBUS3UF1_20930), traffic-NTPase (PilF, TCCBUS3UF1_21340), inner membrane protein (PilC, TCCBUS3UF1_8100), PilM-homolog and secretin-like protein (PilQ, TCCBUS3UF1_6320) were also identified. In addition, genes encoding competence proteins ComZ (TCCBUS3UF1_870), PilN (TCCBUS3UF1_6350), PilO (TCCBUS3UF1_6340), and PilW (TCCBUS3UF1_6330) were present in the chromosome of CCB_US3_UF1. The genes encoding PilM, PilN, PilO, PilW, and PilQ are found to cluster together in the genome (Fig. 4). The rearrangement of these genes is different in Thermus sp. CCB_US3_UF1 compared to T. thermophilus HB27, HB8 and T. scotoductus SA-01, demonstrating the loss of synteny between CCB_US3_UF1 and the other Thermus bacteria. The involvement of Thermus pili in DNA uptake has yet to be determined.
Genomic islands
Potential genomic islands present in the Thermus sp. CCB_US3_UF1 genome were predicted using the IslandViewer database [41]. Early studies on genomic islands focused on regions that carry virulence factors and they are termed pathogenicity islands. Genomic islands are also shown to carry various types of genes associated with many metabolic pathways or biological processes [42]. A total of 11 possible genomic islands were identified in the Thermus sp. CCB_US3_UF1 genome. Several of these genomic islands carry genes encoding proteins involved in transport systems and defense mechanisms. For example, genomic islands 2, 3, 6 and 7 contain numerous transporter genes that may be involved in membrane transport in Thermus sp. CCB_US3_UF1. It is interesting to note that CRISPR-associated Cas proteins that are associated with phage immunity are present on Genomic Island 8 (245986 - 276477) and Genomic Island 10 (1323615 - 1334721). In comparison with other members of Thermus , T. thermophilus HB27 harbors 10 genomic islands while both T. thermophilus HB8 and T. scotoductus SA-01 carry 13 genomic islands.
CRISPR
CRISPR is an RNAi-like system that provides adaptive immunity against phages or other infections is present in prokaryotes [43]. Using the CRISPR Finder tool [44], eight CRISPR repeat regions were detected in the Thermus sp. CCB_US3_UF1 genome (Table 6). The number of spacers in each of these loci are 3, 17, 14, 23, 18, 9, 12, and 2 respectively, i.e. a total of 98 spacers.
A comparison with other Thermus sp. revealed that a total of 10, 11 and 3 CRISPRs were found in T. thermophilus HB27, HB8 and T. scotoductus SA-01, respectively. In terms of the number of spacers, T. thermophilus HB8 has the largest (112), followed by Thermus sp. CCB_US3_UF1 (98), T. scotoductus SA-01 (87) and T. thermophilus HB27 (74). The existence of a large number of CRISPRs in the Thermus genomes reflects an adaptation strategy employed by Thermus to protect themselves from foreign DNA invasion from the surrounding environments.
Isoprenoid biosynthesis
Based on the genome information, Thermus sp. CCB_US3_UF1 synthesizes precursors for isoprenoid compounds from pyruvate and glyceraldehyde 3-phosphate using the deoxyxylulose phosphate (MEP/DOXP) pathway instead of the mevalonate pathway. Isoprenoid compounds are derived from the five-carbon precursor isopentenyl diphosphate (IPP). The genes encoding enzymes of the complete DOXP pathway could be identified in the genome. The DOXP pathway is initiated by the conversion of glyceraldehyde 3-phosphate and pyruvate to 1-deoxy-D-xylulose 5-phosphate (DOXP) catalyzed by DOXP synthase (TCCBUS3UF1_200). Isoprenoid synthesis then proceeds through a series of enzymatic reactions that lead to the formation of 2-C-methyl-D-erythritol-2,4-cyclodiphosphate. Genes encoding the enzymes involved are dxr (TCCBUS3UF1_15410), ispD (TCCBUS3UF1_19830), ispE (TCCBUS3UF1_19820), and ispF (TCCBUS3UF1_380). Genes gcpE (TCCBUS3UF1_18880) and lytB (TCCBUS3UF1_22000), which encode the enzymes involved in the last two steps of isoprenoid synthesis that lead to IPP formation are also encoded in the genome (Additional file 1: Figure S1).
Carotenoid biosynthesis
Most species of the genus Thermus are characterized by the ability to synthesize yellow carotenoid-like pigments [45]. Carotenoids are natural pigments that have been used commercially as food colorants, nutrient supplements and for pharmaceuticals purposes [46]. T. thermophilus has been shown to produce carotenoids known as thermozeaxanthins and thermobiszeaxanthins [47]. As carotenoids are one of the hydrophobic components associated with the cell membrane, it was suggested that carotenoids might have an essential role in stabilizing the membrane of Thermus at high temperature. In T. thermophilus HB27, genes encoding the terminal steps of carotenoid biosynthesis are found in the large plasmid (pTT27), whereas precursor synthesis involving the formation of geranylgeranyl pyrophosphate (GGPP) is accomplished by enzymes encoded on the chromosome [5]. In Thermus sp. CCB_US3_UF1, genes encoding the enzymes for both the terminal and precursor steps of carotenoid biosynthesis are located on the chromosome (Additional file 2: Figure S2).
In the bacterial carotenoid biosynthetic pathway, phytoene is the first carotenoid synthesized and it is formed from the condensation of two molecules of geranylgeranyl pyrophosphate (GGPP) [48]. The GGPP synthase gene (TTHA0013) from T. thermophilus HB8 has been identified and functionally characterized [49]. The gene has a homolog (TCCBUS3UF1_18840) in Thermus sp. CCB_US3_UF1. Phytoene is synthesized from GGPP by phytoene synthase (CrtB). In T. thermophilus HB27, a gene encoding a homolog of phytoene synthase (TT_P0057) was cloned and identified as crtB. It was suggested that phytoene synthase is the rate-limiting enzyme in the carotenoid biosynthesis in T. thermophilus . In addition, crtB of T. thermophilus was found to cluster together with other carotenogenic genes on the large plasmid [50]. Interestingly, the homolog of crtB (TCCBUS3UF1_10160) in Thermus sp. CCB_US3_UF1 is encoded on the chromosome and not the plasmid. Phytoene is then converted to lycopene via a series of desaturation steps that are catalyzed by phytoene desaturase (CrtI), cis-carotene isomerase (CrtH) and ζ-carotene desaturase [51]. In Deinococcus-Thermus bacteria, only one phytoene desaturase, CrtI, has been detected. A gene encoding a CrtI homolog (TCCBUS3UF1_10090) is detected in the genome of Thermus sp. CCB_US3_UF1 as well [5, 52]. Following lycopene synthesis, the carotenoid biosynthetic pathway branches into acyclic and cyclic carotenoids formation. A possible gene encoding an enzyme that catalyzes the cyclization of lycopene, CrtY-type lycopene cyclase (TCCBUS3UF1_10120) is found in the genome of Thermus sp. CCB_US3_UF1 and the other three sequenced Thermus genomes [52] (Additional file 2: Figure S2).
Conclusion
Thermus have proven to be useful as sources of thermostable enzymes and the genome sequences provide information for further exploring the biotechnological potentials of this genus. Analysis of the Thermus sp. CCB_US3_UF1 genome revealed that it encodes pathways for the synthesis of secondary metabolites (isoprenoid) and pigments (carotenoid). The latter has attracted industrial interest for application in food industries. The CRISPR/ Cas system that is found in Thermus could be an interesting tool in molecular biology, particularly for genome editing. Considering the great potential of Thermus in various fields, the complete genome sequence of Thermus sp. CCB_US3_UF1 is a valuable resource for both fundamental researches and biotechnological applications.
Abbreviations
- CCB:
-
Centre for chemical biology
- TEDA:
-
Tianjin economic-technological developmental area
- ATCC:
-
American type culture collection
- CRISPR:
-
Clustered regularly interspaced short palindromic repeats
- BWA:
-
Burrows-wheeler alignment
- USM:
-
Universiti Sains Malaysia
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Acknowledgements
We would like to gratefully acknowledge the help of Dr. Rashidah Abdul Rahim and Muhd Izar bin Omar for isolating the pure culture of Thermus sp. CCB_US3_UF1. This work was partially supported by USM funding 1001/PCCB/870009 to the Centre for Chemical Biology, Universiti Sains Malaysia. This paper is dedicated to our mentor and colleague Maqsudul Alam, in memory of his contributions to genome science.
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Authors’ contributions
MA and NN conceived the project. SH and XW performed library preparation, genome sequencing and assembly. AYAR worked on genome annotation. BST and FLN performed pathway analysis. BST worked on genome analysis and comparative genomics. NSL, JAS and AHT were involved in editing and critical revision of the manuscript. BST prepared and wrote the manuscript. All authors read and approved the final manuscript.
Maqsudul Alam, deceased.
Additional files
Additional file 1: Figure S1.
Metabolic pathway reconstruction of isoprenoid biosynthesis. (TIFF 2139 kb)
Additional file 2: Figure S2.
Metabolic pathway reconstruction of carotenoid biosynthesis. (TIFF 2137 kb)
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Teh, B.S., Lau, NS., Ng, F.L. et al. Complete genome sequence of the thermophilic Thermus sp. CCB_US3_UF1 from a hot spring in Malaysia. Stand in Genomic Sci 10, 76 (2015). https://doi.org/10.1186/s40793-015-0053-6
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DOI: https://doi.org/10.1186/s40793-015-0053-6