Recently, we reported the purification and characterization of three distinct lantibiotics (named suicin 90-1330, suicin 3908, and suicin 65) produced by Streptococcus suis. In this study, we investigated the distribution of the three suicin lantibiotic gene clusters among serotype 2 S. suis strains belonging to sequence type (ST) 25 and ST28, the two dominant STs identified in North America. The genomes of 102 strains were interrogated for the presence of suicin gene clusters encoding suicins 90-1330, 3908, and 65. The gene cluster encoding suicin 65 was the most prevalent and mainly found among ST25 strains. In contrast, none of the genes related to suicin 90-1330 production were identified in 51 ST25 strains nor in 35/51 ST28 strains. However, the complete suicin 90-1330 gene cluster was found in ten ST28 strains, although some genes in the cluster were truncated in three of these isolates. The vast majority (101/102) of S. suis strains did not possess any of the genes encoding suicin 3908. In conclusion, this study indicates heterogeneous distribution of suicin genes in S. suis.
MAPAQWellcome Trust1. Introduction
Bacteriocins are cationic bactericidal peptides that primarily act by disrupting the cell membrane integrity of the target bacteria [1]. More specifically, lantibiotics are an important family of heat stable low molecular weight bacteriocins that possess unusual posttranslationally modified amino acids, such as lanthionine, methyllanthionine, dehydroalanine, and dehydrobutyrine with thioether linkages [2]. Nisin A, produced by Lactococcus lactis subsp. lactis and so far the most studied lantibiotic, was approved as GRAS (Generally Recognized As Safe) by the US Food and Drug Administration (FDA) in 1988 and is currently used commercially in more than 50 countries as a food preservative, especially for dairy products [3]. The lantibiotic biosynthesis machinery involves many enzymes which are encoded by genes organized in gene clusters. Typically, lantibiotic gene clusters include a structural gene encoding a prelantibiotic peptide, as well as genes required for the modification of amino acids, maturation, export, regulation, and immunity [2]. More specifically, the structural gene encodes a prepeptide containing a leader sequence at the N-terminus, which is ultimately cleaved, and a propeptide at the C-terminus in which many or all of the serine and threonine residues are modified [2].
Streptococcus suis is a major swine pathogen responsible for a wide array of infections including life-threatening meningitis, septicemia, and pneumonia [4]. In addition, the organism is an emerging agent of zoonotic disease, particularly in some Asian countries where the general population is at risk [5]. Of the 35 serotypes (1 to 34 and 1/2) that have been originally described based on the composition and structure of the capsular polysaccharides, serotype 2 is the most frequently associated with disease [4, 6]. In the last decade, other serotypes with particular geographical distributions have also been identified as the source of many infections [6]. For instance, in North America, serotypes 2 and 3 show a prevalence of 24.3% and 21%, respectively, followed by serotypes 1/2, 8, and 7 [6]. S. suis serotype 2 can be genotyped using multilocus sequence typing (MLST) [7]. In North America, three genotypes have been described among S. suis serotype 2 strains; the relatively frequent sequence type (ST) 25 and ST28 and the less frequent ST1 [8]. Animal infection models have shown that strains belonging to ST1 are highly virulent whereas ST25 and ST28 isolates have an intermediate and low virulence, respectively [8].
Recently, we purified and characterized three different lantibiotics, named suicins, produced by three distinct strains of S. suis serotype 2 [9–11]. The mature peptides corresponding to each suicin showed poor identity (≤24%) between each other, thus indicating that they are unrelated. Suicin 90-1330 (SslA) is a type A (linear) lantibiotic secreted by a nonvirulent (in both mouse and pig infection models) isolate of S. suis (strain 90-1330) belonging to ST28 and exhibits high homology (90.9%) with nisin U produced by Streptococcus uberis [9]. The production of suicin 90-1330 involves a gene cluster comprising eleven genes [9]. Suicin 3908 (SuiA) is a type B (N-terminal linear and C-terminal globular moieties) lantibiotic produced by a nonvirulent (newborn germ-free pig infection model) isolate of S. suis (strain 3908; unknown ST) isolated from a healthy carrier pig, and shows some identity with bovicin HJ50 (Streptococcus bovis; 49.2% identity) [10]. The suicin 3908 gene cluster contains nine genes [10]. Lastly, a second type B lantibiotic (suicin 65; SssA) showing a high identity with lantibiotics produced by Streptococcus pyogenes (streptococcin FF22, 84.6% identity) and L. lactis subsp. lactis (lacticin 481, 74.1% identity) was identified and characterized in S. suis 65, an ST28 avirulent (newborn germ-free pig infection model) strain isolated from a healthy carrier pig [11]. The gene cluster involved in the production of suicin 65 was found to contain ten genes, including a duplication of the structural gene. Since all three suicins were found to be bactericidal for highly virulent ST1 strains of S. suis [9–11], the use of the purified lantibiotics or the lantibiotic-producing strains may represent a valuable strategy to control S. suis infections and for reducing antibiotic use in the swine industry and consequently the spread of antibiotic resistance. However, the prevalence of the different suicin gene clusters among the circulating population of S. suis strains is not known. In this study, we investigated the distribution and genetic diversity of suicin gene clusters in S. suis serotype 2 belonging to ST25 and ST28, the two dominant STs found in North America.
2. Materials and Methods2.1. Bacterial Strains
One hundred and two strains of S. suis serotype 2 belonging to either ST25 (n=51) or ST28 (n=51) were included in this study (Table 1). These strains were isolated from diseased pigs in Canada, the United States, Japan, and Thailand and have been described previously [12, 13].
Presence and absence of suicin regions and genes among S. suis serotype 2 strains of ST25 and ST28.
Strain
Sequence type
Suicin 65
Suicin 90-1330
Suicin 3908
Present or absent
Number of contigs
Present or absent
Number of contigs
Present or absent
Number of contigs
NSUI001
25
Mostly presenta
1
Absent
N/A
Absent
N/A
NSUI006
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI012
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI033
25
Presentb
1
Absent
N/A
Absent
N/A
NSUI034
25
Present
1
Absent
N/A
Absent
N/A
NSUI035
25
Present
2
Absent
N/A
Absent
N/A
NSUI037
25
Present
1
Absent
N/A
Absent
N/A
NSUI038
25
Present
1
Absent
N/A
Absent
N/A
NSUI039
25
Present
1
Absent
N/A
Absent
N/A
NSUI040
25
Present
1
Absent
N/A
Absent
N/A
NSUI041
25
Mostly present
2
Absent
N/A
Absent
N/A
NSUI042
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI043
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI044
25
Mostly present
2
Absent
N/A
Absent
N/A
NSUI045
25
Mostly present
2
Absent
N/A
Absent
N/A
NSUI046
25
Mostly present
2
Absent
N/A
Absent
N/A
NSUI047
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI048
25
Present
1
Absent
N/A
Absent
N/A
NSUI049
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI050
25
Absentc
N/Ae
Absent
N/A
Absent
N/A
NSUI051
25
Absent
N/A
Absent
N/A
Absent
N/A
NSUI052
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI053
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI054
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI055
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI056
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI057
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI060
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI061
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI063
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI065
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI066
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI068
25
Mostly present
2
Absent
N/A
Absent
N/A
NSUI069
25
Present
1
Absent
N/A
Absent
N/A
NSUI070
25
Present
1
Absent
N/A
Absent
N/A
NSUI072
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI075
25
Mostly present
3
Absent
N/A
Absent
N/A
NSUI077
25
Present
1
Absent
N/A
Absent
N/A
NSUI078
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI082
25
Absent
N/A
Absent
N/A
Absent
N/A
NSUI088
25
Present
1
Absent
N/A
Absent
N/A
NSUI089
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI092
25
Present
1
Absent
N/A
Absent
N/A
NSUI093
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI094
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI096
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI097
25
Present
2
Absent
N/A
Absent
N/A
NSUI099
25
Present
1
Absent
N/A
Absent
N/A
NSUI100
25
Mostly present
3
Absent
N/A
Absent
N/A
NSUI102
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI103
25
Mostly present
1
Absent
N/A
Absent
N/A
NSUI002
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI003
28
Absent
N/A
Present
1
Absent
N/A
NSUI004
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI005
28
Absent
N/A
Present
1
Absent
N/A
NSUI007
28
Absent
N/A
Present
2
Absent
N/A
NSUI008
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI009
28
Absent
N/A
Present
1
Absent
N/A
NSUI010
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI011
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI013
28
Some genesd
N/A
Absent
N/A
Absent
N/A
NSUI014
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI015
28
Absent
N/A
Present
1
Absent
N/A
NSUI016
28
Absent
N/A
Present
1
Absent
N/A
NSUI017
28
Absent
N/A
Present
1
Absent
N/A
NSUI018
28
Absent
N/A
Mostly present
1
Absent
N/A
NSUI019
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI020
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI021
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI022
28
Absent
N/A
Mostly present
2
Absent
N/A
NSUI023
28
Absent
N/A
Mostly present
2
Absent
N/A
NSUI024
28
Absent
N/A
Mostly present
2
Absent
N/A
NSUI025
28
Absent
N/A
Present
2
Absent
N/A
NSUI026
28
Absent
N/A
Mostly present
1
Absent
N/A
NSUI027
28
Present
1
Absent
N/A
Absent
N/A
NSUI028
28
Present
1
Absent
N/A
Absent
N/A
NSUI029
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI030
28
Present
1
Absent
N/A
Absent
N/A
NSUI031
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI032
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI036
28
Absent
N/A
Mostly present
1
Mostly present
1
NSUI058
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI059
28
Present
1
Absent
N/A
Absent
N/A
NSUI062
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI064
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI067
28
Present
1
Absent
N/A
Absent
N/A
NSUI073
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI074
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI076
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI079
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI080
28
Absent
N/A
Present
3
Absent
N/A
NSUI081
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI083
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI084
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI085
28
Present
1
Absent
N/A
Absent
N/A
NSUI086
28
Present
1
Absent
N/A
Absent
N/A
NSUI087
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI090
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI091
28
Absent
N/A
Present
1
Absent
N/A
NSUI095
28
Present
2
Absent
N/A
Absent
N/A
NSUI098
28
Absent
N/A
Absent
N/A
Absent
N/A
NSUI101
28
Absent
N/A
Absent
N/A
Absent
N/A
aThe majority of the genes are present, but some are missing or truncated.
bThe suicin gene cluster is present in its entirety.
cThe suicin gene cluster is completely absent.
dThe majority of the genes are absent, but some are still present.
eN/A: not applicable.
2.2. Genome Analysis
The genomes of the 102 strains were sequenced as paired-end reads with either a HiSeq 2500 or a MiSeq instrument (Illumina, San Diego, CA, USA) as described in previous reports [12, 13]. Sequences with accession numbers SRP065686 and SRP058193, for ST25 and ST28 strains, respectively, were retrieved from the NCBI sequence read archive (SRA). The A5 pipeline was used for de novo assembly of Illumina sequenced strains [14]. Contigs were ordered relative to the reference genome NSUI060 (accession number: CP012911) or NSUI002 (accession number: CP011419), for ST25 and ST28, respectively, using Progressive Mauve [15]. Pseudochromosomes were next created by concatenating the ordered contigs using the sequence NNNNNCATTCCATTCATTAATTAATTAATGAATGAATGNNNNN, which introduces start and stop codons in all 6 reading frames, as a separator. Pseudochromosomes and the genome sequences of reference strains NSUI002 and NSUI060 were converted into queryable BLASTN databases using BLAST+. Gene clusters encoding suicins 90-1330 (accession number: KU867866), 3908 (accession number: KU867867), and 65 (accession number: KU867868) have been described previously and are illustrated in Figure 1 [9–11]. The sequences of individual genes, as well as the full regions for each suicin cluster, were blasted against each genome and pseudochromosome database to test for the presence of genes encoding suicins 90-1330, 3908, and 65. The presence of putative promoter sequences upstream the genes coding for immunity proteins was analyzed with the bacterial promoter recognition program BProm (http://linux1.softberry.com) [16].
Genetic organization of the suicin 90-1330 (a), 3908 (b), and 65 (c) gene clusters. sslA/suiA/sssA/sssA′/sssA1: suicin precursor; sslB: dehydratase involved in suicin synthesis; sslC: cyclase involved in suicin synthesis; sslE/suiE/sssE, sslF/suiF/sssF, sslG/suiG/sssG, and sslI/suiI: immunity proteins; sslK/suiK/sssK: sensor histidine kinase; suiM/sssM: synthetase involved in lantibiotic modification; sslP: protease involved in proteolytic cleavage of the leader peptide; sslR/suiR/sssR: response regulator; sslT/suiT/sssT: ABC transporter.
2.3. Plate Diffusion Assay for Detecting Suicin Susceptibility
Overnight cultures of the suicin-producing S. suis strains (90-1330, 3908, and 65) were spotted (2 μL) on Todd-Hewitt broth (THB; BD-Canada, Mississauga, ON, Canada) agar plates. After a 24 h incubation at 37°C to allow growth, the plates were overlaid with soft THB agar (0.75% agar, w/v) that had been inoculated (700 μL of culture/7 mL of agar) with a 24 h culture of S. suis NSUI018 (possessing immunity gene for suicin 90-1330), NSUI036 (possessing immunity gene for suicin 3908), and NSUI060 (possessing immunity gene for suicin 65). The plates were further incubated for 24 h at 37°C, and the presence of an inhibitory zone was observed.
3. Results and Discussion
Suicin 90-1330 was originally identified in S. suis strain 90-1330, which belongs to ST28 [9]. Interestingly, 35 out of 51 ST28 strains analyzed did not possess any of the genes involved in the production of this suicin (Figure 2). On the other hand, all genes expected in a complete suicin 90-1330 gene cluster were identified in ten ST28 strains, while the locus was partially present in six ST28 strains. However, it is worth mentioning that a full, uninterrupted suicin 90-1330 gene cluster was identified in only seven of these ten ST28 strains (i.e., all genes were identified as a continuum of genes similar to that of Figure 1 in a single contig of the de novo assembled genomes). On the other hand, in one of the ST28 strains that had all suicin 90-1330 genes, the genes were spread across 3 contigs, suggesting two transposon insertions in intergenic regions of the suicin 90-1330 gene cluster. In two other ST28 strains, genes were spread across two contigs, apparently by insertion of a transposon that truncated parts of gene sslT (one strain) or gene sslC (one strain). These transposon insertions should result in strains that are unable to express the suicin. In the six strains in which seven or more suicin 90-1330 cluster genes were only partially present (Figure 2), the gene specifically encoding the structural suicin (sslA) was missing, suggesting that this suicin cannot be produced by these strains. In addition, in 50% of strains with a partial gene cluster, the genes were spread across two contigs (Table 1), probably due to transposon insertions. None of the ST25 strains analyzed in this study possessed genes encoding suicin 90-1330 (Figure 2).
Distribution of suicin 90-1330 gene cluster among S. suis serotype 2 strains of ST25 and ST28. sslA: suicin precursor; sslB: dehydratase involved in suicin synthesis; sslC: cyclase involved in suicin synthesis; sslE, sslF, sslG, and sslI: immunity proteins; sslK: sensor histidine kinase; sslP: protease involved in proteolytic cleavage of the leader peptide; sslR: response regulator; sslT: ABC transporter.
Examination of the genome data revealed that none of the ST25 strains possessed the suicin 3908 gene cluster. Similar results were also observed in 50 of the 51 ST28 isolates (Figure 3). One ST28 strain (NSUI036, isolated in Thailand) possessed some of the cluster genes (in a single contig, Table 1) but lacked the first two genes, suiA (structural gene) and suiM, in full and suiT in part.
Distribution of suicin 3908 gene cluster among S. suis serotype 2 strains of ST25 and ST28. suiA: suicin precursor; suiE, suiF, suiG, and suiI: immunity proteins; suiK: sensor histidine kinase; suiM: synthetase involved in lantibiotic modification; suiR: response regulator; suiT: ABC transporter.
The suicin 65 gene cluster was found in its entirety in 15 of the 51 ST25 strains and partially in 33 of the 51 ST25 strains (Figure 4). Only three ST25 strains did not possess any of the genes of the suicin 65 gene cluster. In the 33 ST25 strains that possessed a partial suicin 65 gene cluster, the structural sssA1 gene and gene sssM were always absent, thus suggesting that these strains cannot produce active suicin 65. The majority of ST28 strains (42/51) did not possess any of the suicin 65 cluster genes. However, eight of the 51 strains possessed all cluster genes. One ST28 strain had only the sssK gene, which lies at the extremity of the cluster. Of the ST25 and ST28 strains that contained the partial or full suicin 65 cluster, 81% (ST25) and 88% (ST28) contained all genes in a single contig (Table 1). In two of the ST25 and ST28 strains that had all suicin 65 genes, the genes were spread across 2 contigs (Table 1).
Distribution of suicin 65 gene cluster among S. suis serotype 2 strains of ST25 and ST28. sssA/sssA′/sssA1: suicin precursor; sssE, sssF, and sssG: immunity proteins; sssK: sensor histidine kinase; sssM: synthetase involved in lantibiotic modification; sssR: response regulator; sssT: ABC transporter.
The in silico analysis described above identified strains which possessed a partial suicin locus containing genes encoding the immunity proteins but no gene encoding the structural suicin protein. More specifically, strain NSUI018 possessed immunity protein for suicin 90-1330, strain NSUI036 possessed immunity protein for suicin 3908, and strain NSUI060 possessed immunity protein for suicin 65. The genomes of these three strains were further analyzed for the presence of promoter-like regions upstream of the genes encoding the immunity proteins. This additional analysis revealed the presence of putative promoter sequences upstream of the gene encoding the immunity proteins in all three strains. However, as demonstrated by a plate diffusion assay, all three strains were found to be susceptible to the strain producing the corresponding suicin (data not shown). Incorporation of CaCO3 ruled out the possibility that inhibition could be related to acid production. Thus, putative sequences identified in silico upstream of the immunity genes are not functional promoters or additional factors are required to allow immunity to suicins. With the perspective to use suicin-producing avirulent strains in prophylaxis, such results indicate that the presence of a partial suicin locus containing the immunity genes does not endow a strain with suicin resistance.
4. Conclusions
The gene clusters encoding suicin 65 (mostly in ST25 strains) and, to a lesser extent, suicin 90-1330 (exclusively in ST28 strains) were the most prevalent. None of the strains that had suicin 90-1330 had suicin 65 and vice versa.
Competing Interests
The authors declare that they have no competing interests.
Acknowledgments
This study was supported by a grant from the Ministère de l’Agriculture, des Pêcheries et de l’Alimentation du Québec (MAPAQ). The authors wish to thank G. LeBel for technical assistance. This study made use of the Streptococcus suis Multilocus Sequence Typing Database hosted at Imperial College and whose development is funded by the Wellcome Trust.
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