Whole-genome sequences of multidrug-resistant Escherichia coli in South-Kivu Province, Democratic Republic of Congo: characterization of phylogenomic changes, virulence and resistance genes

The set of 21 ESBL-producing E. coli isolates analyzed in the current study came from a collection of isolates assembled between 2012 and 2014 from inpatients at the Bukavu General Hospital, South Kivu (DRC, see Fig. 1). All isolates were phenotypically identified by standard biochemical tests including oxidase testing, triple sugar iron, imviC tests (Indole, Methyl Red, Voges-Proskaeur, and Citrate utilization), urease and motility.

The susceptibility to 14 antimicrobial agents (i.e. amikacin, amoxicillin, amoxicillin-clavulanic acid, ampicillin, ceftazidime, ceftriaxone, cefepime, cefotaxime, cefuroxime, chloramphenicol, ciprofloxacin, imipenem, trimethoprim-sulfamethoxazole and tetracycline) was determined by the disk diffusion method according to the European Committee on Antimicrobial Susceptibility Testing (EUCAST) guidelines as updated in January 2017 [21]. Minimum Inhibitory Concentrations (MIC) for each of the 15 antimicrobial agents was determined after 16–20 h incubation on Mueller-Hinton plates inoculated with suspensions of isolates at a fixed density (0.5 to 0.6 McFarland standard), using E-test strips (BioMérieux, Marcy l’Etoile, France) according to the manufacturer’s recommendations. Additionally, isolates were tested for ESBL-production by the double-disk synergy method on Mueller-Hinton agar using ceftazidime and ceftriaxone placed at a distance of 20 mm apart from a disk containing amoxicillin plus clavulanic acid. A clear-cut enhancement of the inhibition in front of either ceftazidime and/or ceftriaxone disks towards the clavulanic acid-containing disk (also called “champagne-cork” or “keyhole”) was interpreted as positive for ESBL production [22]. E-test strips (BioMérieux, Marcy l’Etoile, France) were used for confirmation of ESBL production, following the manufacturer’s instructions. E. coli ATCC 35218 and Klebsiella pneumoniae ATCC 700603 strains were used as ESBL-negative and positive controls, respectively. In addition, isolates were tested for the presence of the beta-lactamase AmpC phenotype using cefoxitin-cloxacillin disk diffusion test as described previously [23].

Paired-end reads from each E. coli isolate were assembled de novo using the Spades v.3.11.1 algorithm [24] to generate a draft genome sequence for each isolate and quality assessment for genome assemblies was carried out using QUAST 4.5 [25]. Raw genome data have been submitted to the European Nucleotide Archive (ENA, http://​www.​ebi.​ac.​uk/​ena) and are available under accession number ERS1812814-ERS1812829. MLST typing was performed on draft (n = 21) and on complete genomes of ExPEC from GenBank by using the E. coli MLST scheme developed by Achtman [26] and the home-made Pathogenomic R package (https://​github.​com/​JeromeAmbroise/​Pathogenomics). The latter was used to screen all draft (n = 21) and complete genomes of E. coli sharing the same STs with DRC isolates for the virulence factor genes described in ExPEC [27‐29] and/or available in the Virulence Finder database (https://​cge.​cbs.​dtu.​dk/​services/​VirulenceFinder/​) with a threshold of 95% identity and a minimum length of 80%. Concurrently, each draft genome was screened for the presence of AMR genes. The complete list of screened genes was drawn up from the MEGARes database (https://​megares.​meglab.​org). In order to selectively identify AMR genes acquired through horizontal gene transfer, the list based on MEGARes data was restricted to genes that were also found in the ResFinder database (https://​cge.​cbs.​dtu.​dk/​services/​ResFinder/​), using BLASTn. In addition, SNP-based AMR chromosomal determinants were identified using the ARIBA software [30] with the MEGARes database. Assembled contigs were further assessed for the presence of plasmid replicons using the plasmid multilocus sequence typing (pMLST) database [31]. The F plasmids were further categorized by the FAB (FII, FIA, FIB) formula using the replicon sequence typing (RST) scheme described by Villa [32]. The DNA sequences of novel FIB and FII replicons were submitted to the pMLST database curator (https://​pubmlst.​org/​plasmid/​) for the assignment of the ST. All drafts (n = 21) and ST-relevant complete genomes from GenBank were submitted to kSNP3.0 for SNP identification and Maximum Likelihood phylogenetic tree construction. This software performs SNP identification without genome alignment nor requirement for reference genomes. In parallel, WGS data were used to characterize E. coli isolates through the combination of four DNA gene markers (i.e. ArpA, chuA, yjaA and TSPE4-C2) as described by Clermont et al. [33]. In brief, E. coli draft genomes were screened for the presence of these four genetic markers, a combination thereof determining the phylogenetic clustered distribution of the isolates. Those isolates which belong to the B2 phylogenetic group were further screened for the ST131-O25b clone-specific silent SNPs in the E. coli pabB gene (C267T and G573A, accession number: CP015085) as previously described [34].

All isolates (n = 21) were MDR ESBL-producing E. coli (Fig. 2). MIC data are provided in in Table 1. The majority of isolates displayed low susceptibility to amoxicillin, amoxicillin-clavulanic acid, ampicillin, ceftazidime, cefuroxime, ceftriaxone, cefotaxime, chloramphenicol, ciprofloxacin, imipenem, trimethoprim-sulfamethoxazole and tetracycline. In contrast, all and 19/21 DRC E. coli isolates were susceptible to imipenem and amikacin, respectively.

Computation of the total number of reads and quality metrics of the assemblies (Additional file 1) showed homogenous results with a good quality profile for all isolates.

E. coli isolates (n = 21) were clustered into three major clades (Fig. 3). The first one grouped seven ST131 ExPEC isolates (DRC_BKV_03, DRC_BKV_04, DRC_BKV_05, DRC_BKV_12, DRC_BKV_13, DRC_BKV_14, and DRC_BKV_16), one ST95 isolate (DRC_BKV_19), and one ST648 isolate (DRC_BKV_20). All ST131 isolates belonged to the same sub-clade and to the phylogenetic group B2 according to Clermont et al. [33]. All displayed the C267T and the G573A substitutions in the pabB gene in line with their O25b-ST131 status [34] (Fig. 3). The second clade included seven isolates belonging to unrelated various STs (i.e., DRC_BKV_01: ST617; DRC_BKV_08: ST10; DRC_BKV_15: ST2450; DRC_BKV_17 and DRC_BKV_21: ST410; DRC_BKV_11: ST58; DRC_BKV_18: ST443).

The third clade contained four ST405 isolates (i.e., DRC_BKV_06, DRC_BKV_07, DRC_BKV_09, and DRC_BKV_10), and one ST393 isolate (DRC_BKV_02).

At first sight, virulence factors identified in DRC ST131 E.coli isolates are similar to those reported in pandemic CTX-M-15-producing E. coli O25b-ST131 [28, 35‐37]. However, E. coli O25-b-ST131 from DRC harbored significantly (p < 0.01, t-test) more virulence genes (Fig. 4) as illustrated by the presence of the traT gene carried by all but one (DRC_BKV_12) DRC E.coli O25b-ST131. This gene was not detected in any of the E. coli genomes selected from Genbank (Fig. 4). Likewise, two out of 7 DRC O25b-ST131 isolates (i.e., DRC_BKV_04 and DRC_BKV_05) harbored the ireA virulence gene, which was absent from similar strain sequences in GenBank [35]. DRC ST131 E. coli were mostly (5/7) isolated from bloodstream and, as expected, harbored more virulence genes than DRC ST405 E. coli. The latter isolates were mostly (3/4) isolated from urine.

Each draft genome sequence of ExPEC isolates from South Kivu harbored AMR genes. They consisted in chromosomal SNP-based determinants of AMR and/or plasmid-mediated AMR to various classes of antibiotics (Additional file 2 and Fig. 5). Some chromosomal SNP-based determinants of AMR corresponded to amino acid substitutions leading to resistance to several antibiotics, e.g. quinolones, sulfonamides, rifampicin, and elfamycins. Other chromosomal SNP-based determinants of AMR caused amino acids substitutions in several MDR genes (OMPF porin, PhoP multi-drug efflux pump) [38] and/or in genes which regulate the expression of several AMR genes, such as MARR (Multiple Antibiotic Resistance Regulator) and soxS (a member of Superoxide regulon) [39]. Analysis of MIC values for ciprofloxacin revealed that, whereas all DRC E. coli isolates were resistant to ciprofloxacin, high level resistance to this drug was overall associated with amino acid substitutions in quinolone-resistance-determining-regions (QRDR) of gyrA gene (S83 L, D87N) and/or in QRDR of parC gene (S80I, E84V, S57T, E84G). In addition, several SNPs resulting in amino acid substitutions were also characterized in gyrB and parE genes. Noticeably, none of these substitutions occurred in the respective QRDRs of both latter genes. These findings are consistent with other studies emphasizing the importance of substitutions in QRDRs of gyrA and parC proteins in the emergence of high level resistance to quinolones [40, 41]. However, given the limited set of data analyzed in this study, a confirmation of the role played by chromosomal SNP-based determinants in the emergence of quinolone resistance in DRC isolates requires further assessment.

The CTX-M-15 gene, which encodes a protein responsible for the ESBL phenotype, was detected in all but one isolate (DRC_BKV_01). WGS-based analysis identified plasmid replicons in 21/21 isolates. Beside well-characterized alleles, RST revealed the presence of three new plasmid replicons, FIB 69 FII 105 and FII 107, which are reported here for the first time. Twelve different RST profiles were characterized in the 22 plasmid replicons: F105:A1:B69 (DRC_BKV_06, DRC_BKV_07, DRC_BKV_09, and DRC_BKV_10), F31:A4:B1 (DRC_BKV_01, DRC_BKV_08, and DRC_BKV_16), F48:A1:B49 (DRC_BKV_04 and DRC_BKV_05), F1:A2:B20 (DRC_BKV_13 and DRC_BKV_14), F2:A-:B1 (DRC_BKV_11 and DRC_BKV_15), F1:A1:B1 (DRC_BKV_18 and DRC_BKV_20), F1:A1:B16 (DRC_BKV_12), F36:A1:B1 (DRC_BKV_02), F1:A1:B49 (DRC_BKV_17), F107:A-:B:1 (DRC_BKV_19), F2:A1:B1 (DRC_BKV_21), and F1:A:2:B- (DRC_BKV_03). It is noteworthy that, except for IncF, no other incompatibility plasmid replicon types (i.e., IncA/C, IncH1, IncH2, IncI1, and IncN) were identified in these DRC isolates.