A clinical strain of S. agalactiae, Sag37, was isolated from the blood sample of a new-born with bacteremia in Shanghai in 2014. Another clinical strain of S. agalactiae, Sag158, was isolated from the blood sample of another new-born, and was used as the recipient. The minimum inhibitory concentrations (MICs) of erythromycin, tetracycline, levofloxacin, clindamycin, and penicillin were determined using the Etest (bioMe’rieux, France), and the results were interpreted based on the guidelines of the Clinical and Laboratory Standards Institutes [CLSI] (2014).

Multilocus sequence typing analysis (MLST) and serotyping was performed as previously described (Jones et al., 2003; Imperi et al., 2010). After MLST, an online database¹ was used for assigning allele numbers, and the sequence types (STs) were obtained from the combination of the results.

Conjugal transfer experiments were performed in broth culture using the strain Sag37 (erythromycin-resistant and levofloxacin-susceptible) as the donor and the strain Sag158 (erythromycin-susceptible and levofloxacin-resistant) as the recipient. Briefly, donor and recipient strains were grown to an OD₆₀₀ of 0.4 and mixed in a ratio of 1:1 in 2 ml of culture. The suspension was pelleted, resuspended, and used for mating. Selection was performed with suitable concentrations of erythromycin (1 mg/L) and levofloxacin (8 mg/L). All transfer experiments were performed at least thrice. Sag158 and the transconjugant, Sag158-1, were both digested with SmaI endonuclease and S1 nuclease and subjected to PFGE and S1-PFGE, as described in previous studies (Barton et al., 1995; Elliott et al., 1998). Briefly, two or three colonies were selected from a fresh plate of overnight growth and incubated in Todd-Hewitt broth for 5 h at 35°C; this suspension was centrifuged and the pellet was re-suspended in Tris–NaCl buffer. The agarose-bacterium plugs were generated and incubated overnight at 35°C in lysis solution. The plugs were washed several times and digested with a suitable nuclease. The chromosomal digests were separated by PFGE. Pulsotypes were clustered based on a cut-off of 70% similarity.

The genomic DNA was extracted using the QIAGEN Midi Kit (Qiagen, Hilden, Germany). The DNA of Sag37 and Sag158 was sequenced using the pacbio RS II (Pacific Biosciences, Menlo Park, CA, United States). The reads were de novo assembled using the HGAP 3.0 SMRT^TM Pipe. The transconjugant was sequenced using the illumina HiSeq sequencing approach. SOAP de novo² was used to perform genome assembly. Sequence similarity searches were carried out using BLAST³. Open reading frames (ORFs) were predicted using the ORF Finder software⁴. Protein-coding genes were initially identified and annotated using RAST. The antimicrobial resistance genes were identified using ResFinder⁵.

PCR assays were performed with three pairs of primers (Table 1), rumAF and SR; rumAR and EF; and rumAF and rumAR (Figure 1), to confirm its site-specific integration: rumA. Outward-directed primers (SR and EF) were used to detect the circular form of ICESag37. DNA preparation, amplification, and electrophoresis of the PCR products were carried out by previously established procedures (Hynes et al., 1992) in conditions indicated for the use of individual primer pairs. The PCR products were verified by sequencing.

The nucleotide sequences of Sag37 and Sag158 have been deposited in the Genbank sequence database under the accession numbers CP019978 and CP019979, respectively. The sequence read archive (SRA) of Sag158-1 has been deposited in Genbank under the accession number SRR5585701.

Sag37 was highly resistant to erythromycin, clindamycin, and tetracycline and susceptible to levofloxacin and penicillin, while Sag158 was resistant to tetracycline and levofloxacin, and susceptible to erythromycin, clindamycin, and penicillin. Sag37 and Sag158 displayed different STs (12 and 19, respectively) and serotypes (Ib and III, respectively). All these results, the isolation data, and the resistance genes of the two strains are summarized in Table 2.

Through mating experiments, erythromycin resistance was transferred from the donor, Sag37 (erythromycin-resistant and levofloxacin-susceptible), to the recipient, Sag158 (erythromycin-susceptible and levofloxacin-resistant), at a frequency of ∼3 × 10^-7. Randomly selected erythromycin-resistant transconjugants were used for further experiments. The principle features and MICs of the transconjugant, Sag158-1, are summarized in Table 1. Sag158-1 showed the same erythromycin MIC as the donor and a higher tetracycline MIC than the donor strain. SmaI-PFGE analysis indicated a new SmaI fragment (Figure 2). S1-PFGE revealed that Sag37 harbored no plasmids. The erythromycin resistance was also transferred from Sag37 to two other clinical S. agalactiae recipients, although the data is not shown in this paper.

Whole genome sequencing was carried out for the two strains investigated in this study, Sag37 and Sag158. The genomes of Sag37 and Sag158 comprised a single circular chromosome and were 2,198,785 and 2,096,882 bp in length, respectively, with average G + C contents of 35.77 and 35.66%, respectively. A total of 2180 protein coding sequences (CDS) were predicted in Sag37, while 2093 CDS were predicted in Sag158. Different substitutions were found in the quinolone resistance-determining regions of Sag158 (Ser81Leu in gyrA and Ser79Tyr and Ser140Pro in parC), which were not found in Sag37.

In order to track possible genomic clues regarding the mobile elements, comparative genome analyses were performed for Sag37, Sag158, and Sag158-1. We identified a contig in Sag158-1, which contained all the resistance genes that were present in Sag37, but were absent in Sag158. We aligned this contig with Sag37 and Sag 158, and confirmed that it did exist in Sag37, but was absent in Sag158. Further sequence analysis confirmed the presence of a ∼75-kb mobile element carrying erm(B) and tet(O).

PCR assays using outward-directed primers (SR and EF) revealed that the mobile element could excise and form a covalently circular intermediate in both Sag37 and Sag158-1 (Figure 1). Sequence analysis of the amplicons and the left and right junctions of the mobile element enabled us to identify the putative core sites (attI, attL, and attR) and obtain the complete sequence.

Sequences adjacent to the ends of the mobile element in Sag37 and Sag158-1 suggested a possible integration site. PCR assays with three pairs of primers, rumAF and SR; rumAR and EF; and rumAF and rumAR (Figure 1), and sequence analysis of the amplicons confirmed the site-specific integration. The mobile element encoded a serine family integrase, which mediated chromosomal integration at the 3′ end of the conserved gene, rumA (23S rRNA [uracil-5-]-methyltransferase). The integrase was also confirmed through a PCR assay.

The results of the mating experiments, the PFGE, and the PCR assays provided a glimpse of the mobile element. The results of the whole genome sequencing and the extensive sequence analysis revealed its full picture. It was designated ICESag37 and is schematically represented in Figure 3. ICESag37 was found to be 73,429 kb in size (629058–702486 bp in Sag37) and predicted to contain 79 ORFs. In addition to the serine family integrase, ICESag37 also contained several genes belong to a type IV secretion system (T4SS), as well as genes encoding putative mobilization proteins of the MobC family and relaxases (Figure 1). The transferability of ICESag37, as shown in the conjugation experiments, strongly suggested that it had an intact and feasible transfer system.

ICESag37 carried resistance genes to multiple antibiotics, including erythromycin [erm(B)], tetracycline [tet(O)], and aminoglycosides [aadE, aphA, and ant(6)]. The mosaic genes from the Enterococcus faecalis plasmid, pLG2, were also observed in ICESag37 (Figure 2), and it was this plasmid that introduced the erythromycin resistance determinant, erm(B), as well as the aminoglycoside resistance gene cluster containing ant(6) and aphA, into ICESag37. ISSag12 was integrated into the mosaic genes, disrupting the sat gene. tet(O) and aadE were also embedded in ICESag37, although the source was not known. In addition to the antibiotic resistance genes, ICESag37 also contained genes predicted to be involved in virulence, a two-component signal transduction system (nisK/nisR), from S. suis.