Disease Severity

We considered patients with >1 of the following to have severe GCGS disease: in-hospital death, admission to intensive care unit, need for vasopressor or ventilatory support, diagnosis of streptococcal toxic shock syndrome (STSS) or infectious endocarditis, or a high-risk Simple Clinical Score >8 or Rapid Emergency Medicine Score >10. We defined STSS according to guidelines of the Working Group on Severe Streptococcal Infections (25). We calculated Simple Clinical Scores and Rapid Emergency Medicine Scores primarily by using patient vital signs and other clinical features; high-risk scores are associated with a 9.0%–10.3% risk for death by 30 days after admission (26–28).

Collection and Identification of Bacteria

At the discretion of the healthcare provider, patient blood samples were collected at symptom onset into BacT/Alert bottles (bioMérieux, Saint-Laurent, QC, Canada) according to institutional protocol and incubated using the BacT/Alert blood culture instrument (bioMérieux). Isolates were stored in frozen stocks in skim milk at −70°C and later retrieved by subculture for further analysis.

A total of 92 GCGS isolates were recorded during the study period; 90 were retrieved, 2 were lost in storage, and 1 was identified as S. equi subsp. zooepidemicus by 16S rRNA sequence similarity and excluded from the study. We plated the 89 remaining isolates onto sheep blood agar (Oxoid, Nepean, ON, Canada) and aerobically incubated them for 24 h at 37°C in the presence of 5% CO₂. We confirmed isolate identification by using MALDI-TOF (matrix-assisted laser desorption/ionization time-of-flight) mass spectrometry with the MALDI BioTyper system (Bruker, Boston, MA, USA) according to the manufacturer’s protocol. To confirm isolates with ambiguous MALDI-TOF mass spectrometry identifications, we used latex agglutination to Lancefield antigens C and G and the Vitek2 system (bioMérieux) for biochemical identification. All isolates were identified as S. dysgalactiae.

Whole-Genome Sequencing

We extracted DNA from cultures, created multiplexed libraries, assembled reads, and performed core nucleotide variation phylogenetic analyses (Technical Appendix 1). In brief, we generated paired-end, 300-bp indexed reads on the Illumina MiSeq platform (Illumina, San Diego, CA, USA); the average yield was 1,015,107 reads/genome, and the average genomic coverage was 145×. Read quality was assessed by using FastQC version 0.11.4 (http://www.bioinformatics.babraham.ac.uk/projects/fastqc/), assembled with SPAdes version 3.6.2 (http://cab.spbu.ru/software/spades/), and annotated with Prokka version 1.11 (http://www.vicbioinformatics.com/software.prokka.shtml), yielding an average contig length of 39,313 bp and an average N50 contig length of 82,867 bp (29–31). The high-quality reads were then mapped to the publically available reference genome, S. dysgalactiae subsp. equisimilis AC-2713 (GenBank accession no. NC_019042.1), by using SMALT version 0.7.5 (http://www.sanger.ac.uk/science/tools/smalt-0). Single-nucleotide variations (SNVs) were called using FreeBayes version 0.9.20 (https://github.com/ekg/freebayes) and SAMtools mpileup (http://www.htslib.org/) (32). The percentage of bases in the core was 82.8%, and 21,746 sites were used to generate the phylogeny.

We constructed a maximum-likelihood phylogenetic tree of informative SNV positions by using PhyML version 3.0 (http://www.atgc-montpellier.fr/phyml/) (33) and visualized the tree by using FigTree version 1.4.1 (http://tree.bio.ed.ac.uk/software/figtree/) (34). We determined phylogenetic clades by cluster analysis on the full dataset of blood and respiratory isolates (n = 122) and on isolates from blood only (n = 89) by using ClusterPicker version 1.2.4 (http://hiv.bio.ed.ac.uk/software.html) with the following settings: initial and main support thresholds = 0.9, genetic distance threshold = 4.5, and the large cluster threshold = 10 (34). We submitted whole-genome sequencing read data to the NCBI Sequence Read Archive (https://www.ncbi.nlm.nih.gov/sra/) under BioProject accession number PRJNA325743.

Molecular Typing

We used the whole-genome sequencing data for in silico determination of MLST STs; virulence factors (lmb, gapC, cba, cbp, fbp, sagA, slo, hylB, spegg, sicG, fbsA, pavA, fnbA, fnbB, gfbA, scpA, scpB, bca, cylE, ska, skc and skg) (22,35); and superantigens (speA, speB, speC, speF, spegg, speH, speI, speJ, speL, mf-2, mf-3, and smeZ) (21,23). We determined Lancefield serogroups from sequences annotated with Prokka and confirmed them by serologic testing using commercial latex antisera (SSI Diagnostica, Hillerød, Denmark). We submitted MLST allelic profiles to the Streptococcus dysgalactiae MLST database (https://pubmlst.org/sdysgalactiae/). We used allelic profiles to compute a goeBURST (global optimal eBurst; http://www.phyloviz.net/goeburst/) full minimum spanning tree using PHYLOViZ (http://www.phyloviz.net/) (36); groups were assigned by a single-locus variation from a founding ST. All strains were confirmed to belong to S. dysgalactiae subsp. equisimilis by BLASTn (37) alignment of 16S rRNA sequences to reference genomes of S. dysgalactiae subsp. dysgalactiae ATCC27957 and S. dysgalactiae subsp. equisimilis ATCC12394 (PubMed accession nos. NZ_CM001076.1 and NC_017567.1, respectively).

Statistical Methods

We used descriptive statistics, χ² test, Kruskal-Wallis test, and Fisher exact test to compare demographics between clusters of SDSE to determine whether they differed with respect to key risk factors. We used Fisher exact test to compare risk of death and other disease severity markers between ST clusters and clades. No observations were censored, so survival analysis techniques were not necessary.

Patient Characteristics and Disease Severity

We investigated 89 GCGS bacteremic events in 84 patients in Winnipeg during 2012–2014. Most patients (63%) were male, and the mean age was 61 years (SD ± 18.4 years). Many patients had co-existing conditions, predominantly cardiovascular disease (47%) and diabetes mellitus (43%). The most common source of bacteremia was from skin and soft tissue infections (51%), and 37% of patients had primary bacteremia. Infectious endocarditis was confirmed or suspected in 7% of patients. No patients had necrotizing fasciitis or pharyngitis (Table 1).

In 70% of the cases, bacteremia was associated with markers of severe disease, including admission to an intensive care unit (26%) and the need for vasopressor (19%) or ventilatory (17%) support. Seventeen percent of patients had a diagnosis of STSS, and 35%–61% of patients had high-risk disease severity scores. Twenty percent of patients with GCGS bacteremia died while in the hospital (Table 2).

SDSE Isolate Characteristics

SDSE isolates from blood represented 89 (73%) of 122 total isolates; 33 (37%) of the 89 isolates were from female patients and 56 (63%) were from male patients. These isolates were classified as Lancefield groups G (63%) and C (37%). Respiratory isolates represented 27% (33/122) of the isolates; information regarding the number from female and male patients was not available. These isolates also were classified as Lancefield groups G (52%) and C (48%).

Core Single-Nucleotide Variation Phylogenetic Analysis

Phylogenetic analysis of all 122 isolates showed no association between infection type and patient sex, age, or disease severity (Technical Appendix 1 Figure). Compared with the heterogeneous nonclade isolates, those that clustered into clades A–E represented a higher proportion of blood isolates (25/45 [57%] vs. 64/77 [83%], respectively; p = 0.002). In addition, compared with the other clades combined, clade A was represented by significantly fewer blood isolates (36/38 [95%] vs. 28/39 [72%], respectively; p = 0.017). In silico molecular determinants (MLST, Lancefield serogroups, and virulence factors) were clustered in a clonal distribution (Technical Appendix 1 Figure). However, we found no significant associations when comparing blood and respiratory isolates.

Figure 1

Figure 1. Maximum-likelihood whole-genome, core single-nucleotide variation (SNV) phylogenetic tree of 89 Streptococcus dysgalactiae subsp. equisimilis isolates from the blood of patients with group C and G Streptococcus causing severe infections, Winnipeg,...

Cluster analysis of the 89 blood isolates yielded 5 clades, A–E (n = 64); the other 25 heterogeneous isolates were outside these lineages. Clade A isolates were Lancefield serogroup C, clades B–E were serogroup G, and the heterogeneous nonclade isolates were serogroups C (n = 5) and G (n = 20) (Figure 1). Isolate numbers 35, 49, 26, 40, 47, 45, and 51 were most genetically distant from the other blood isolates, averaging 3,897–3,987 SNVs. The greatest difference was 5,110 SNVs between isolate numbers 30 and 51 (Technical Appendix 2). Clade C was the most genetically homogenous, showing a maximum of 138 SNVs between isolates in the clade. Clade B was the most diverse, showing a maximum difference of 600 SNVs between isolates (online Technical Appendix Table 1).

MLST

Figure 2

Figure 2. Minimum spanning tree representing the genetic relatedness of multilocus sequence types (MLSTs) of Streptococcus dysgalactiae subsp. equisimilis isolates from patients with group C and G Streptococcus causing severe infections, Winnipeg,...

STs for all 122 isolates generally correlated with specific phylogenetic clades and subclades (Figure 1; Technical Appendix 1 Figure). The most common STs were ST20 (n = 28), followed by ST17 (n = 16) and ST15 (n = 9) (Figure 2). Clade A (n = 28) consisted entirely of ST20 isolates belonging to a singleton MLST relatedness group. Clade B (n = 13) belonged to MLST clonal complex (CC) 2, in which ST15 (n = 9), ST69 (n = 1), and ST274 (n = 2) isolates grouped into subclades. An isolate with ST276 (a double-locus variant of ST15) also clustered into clade B. Clades C (n = 14) and D (n = 5) belonged to MLST CC1; clade C consisted of ST17 isolates, and clade D consisted of ST282 isolates. Clade E (n = 4) belonged to MLST CC3, in which ST63 (n = 2), ST52 (n = 1), and ST164 (n = 1) isolates grouped into subclades. Although SNV phylogenetic analysis showed that ST17 (clade C) and ST15 (clade B) isolates were closely related, large variations in MLST separated them into distinct clonal clusters (Figure 2).

Figure 3

Figure 3. Prevalence of sequence types, as characterized by multilocus sequence typing, among blood and respiratory isolates of Streptococcus dysgalactiae subsp. equisimilis from patients with group C and G Streptococcus causing severe...

A total of 18 STs were unique to blood isolates: STs 4, 8, 38, 44, 52, 59, 63, 84, 138, 154, 265, 269, 270, 274, 275, 276, 279, and 282. A total of 8 STs were unique to respiratory isolates: STs 49, 68, 206, 266, 273, 277, 280, and 283 (Figure 3).

Invasive Polymicrobial Infections

Polymicrobial bacteremia with organisms other than GCGS alone was present in 18% (16/89) of patients. In 4 patients with non-GCGS organisms plus GCGS isolates (i.e., isolate nos. 3 and 57, which clustered in clade B; and nonclade nos. 12 and 74), the non-GCGS organisms were believed to represent 1) contaminants at the time of sample collection or 2) the nonprimary pathogen. Staphylococcus aureus co-infection was seen in 6 patients. Four patients had GCGS isolates that clustered into clade C (nos. 41, 70, 82, 85), and the isolates were all associated with severe disease features (Technical Appendix 1 Table 2). Two of the 4 patients died.

Distribution of Virulence Factors

All 122 isolates carried virulence factors gapC, hylB, lmb, sagA, scpA, scpB, ska, skc, skg, and slo; however, virulence factors cba, cfb, cylE, fbsA, fnbA, and pavA were universally absent. Other factors were variably present (Table 3). Factors cbp, fbp, speG, sicG, gfbA, and bca clustered clonally into the phylogeny (Figure 1). All clade A and B isolates contained only speG, with the exception of 1 clade B isolate that also contained cbp, sicG, and gfbA. Clade C consisted of isolates with cbp, sicG, and gfbA; clade D isolates had cbp, fbp, and sicG; and clade E isolates had fbp, speG, and sicG. The virulence factor fbp was present in clades D and E and in 1 nonclade isolate (no. 28). Virulence factor bca was found variably in 5 nonclade isolates (nos. 49, 75, 74, 33, and 11) and in the reference isolate, AC-2713, which also contained genes speG and sicG. No association was discovered between the presence of these virulence factors and disease severity.

Clinical Outcomes within the Phylogeny

Severe disease features were present in a similar proportion of patients with GCGS disease caused by clade A–E isolates (63%, 40/64 patients) and heterogeneous nonclade isolates (68%, 17/25 patients). There was an observed trend toward increased mortality in patients with isolates from clades A–E (14 deaths) compared with patients with nonclade isolates (4 deaths), although the difference was not statistically significant (p = 0.7698). The number of deaths resulting from GCGS bacteremia caused by the most common clades, A–C (13/55 [24%]), was not significantly different than the number caused by other clades (5/34 [15%]; p = 0.4179). The death rate was also higher among patients with ST15, ST20, and ST17 (26% [14/53 patients]) than among patients with other STs (11% [4/36 patients]), but the difference was not significant (p = 0.1075).