We identified AMR determinants (i.e., the mtrR-35A, mtr₁₂₀, and mosaic N. meningitidis–like mtrR mutations) in addition to the MtrR A39T and G45D amino acid mutations in silico from WGS data, as described (26,28). We aligned and compared the mtr locus and rplD, rplV, and macAB sequences with the N. gonorrhoeae FA1090 reference genome (GenBank accession no. AE004969). To identify the frequency of 23S rRNA A2059G and C2611T mutations (named using Escherichia coli numbering), we mapped sequence reads against a single copy of the FA1090 23S rRNA gene using Burrow-Wheeler Aligner version 0.7.17 (http://bio-bwa.sourceforge.net) with the default settings. We determined base counts using a custom script, enabling the estimation of the proportion of copies with the A2059G, C2611T, or both mutations. We examined additional macrolide resistance genes (e.g., ereA, ereB, ermA, ermB, mefA, mefB, msrA, and msrC) using ARIBA version 2.14.4 and the ResFinder (https://cge.cbs.dtu.dk/services/ResFinder) and CARD (https://card.mcmaster.ca) databases (29). We identified alleles in silico from WGS data using N. gonorrhoeae multiantigen sequence typing (NG-MAST), multilocus sequence typing (MLST), and N. gonorrhoeae sequence typing for antimicrobial resistance (NG-STAR). We used the MLST (https://pubmlst.org/neisseria), NG-MAST (http://www.ng-mast.net), and NG-STAR (https://ngstar.canada.ca) databases to assign allele numbers and sequence types (ST)s (30,31). We grouped closely related NG-MAST STs using a previously described genogroup definition (28).

For phylogenetic analysis, we identified single-nucleotide polymorphisms (SNPs) in sequence reads mapped against the WHO P reference genome using the variant calling tool Snippy version 4.4.5 (https://github.com/tseemann/snippy). We identified and filtered recombinant regions using Gubbins version 2.1.0 (Sanger, https://sanger-pathogens.github.io/gubbins); the resulting core SNP alignment consisted of 9,415 sites. We used IQ-tree version 1.6.1 (http://www.iqtree.org) to infer a maximum-likelihood tree from the whole-genome SNP alignment with a generalized time-reversible model of evolution using gamma correction for among-site rate variation with 4 rate categories; branch support was estimated by bootstrap analysis of 10,000 replicates (32). We visualized the resulting phylogeny with Figtree version 1.4.4 (http://tree.bio.ed.ac.uk/software/figtree) and phandango (33). We clustered sequences using RAMI with a branch length threshold of 0.01 (34). For comparison, we selected international isolates and publicly available genomic data on the basis of MICs, MLST STs (i.e., ST9363 and ST1580), and NG-MAST genogroups (i.e., G470 and G12302) from the National Center for Biotechnology Information (https://www.ncbi.nlm.nih.gov), European Molecular Biology Laboratory (https://www.embl.org), and the DNA Data Bank of Japan (https://www.ddbj.nig.ac.jp). We found 17 genomes from the United Kingdom, 3 from Canada, 3 from Scotland, 17 from Australia, 28 from the United States, 7 from Brazil, and 11 from Norway (16,17,24,25,35–37). We generated a phylogenetic tree of 86 international and 96 isolates from Argentina as described for domestic isolates and visualized the tree in Figtree version 1.4.4. Sequence reads are available from the European Nucleotide Archive (accession no. PRJEB41007).

The 96 N. gonorrhoeae isolates were collected from male (90.6%) and female (6.3%) patients; sex was unreported for 3.1% of patients. Patient age was reported for 88 (91.7%) isolates. Patients were 4–47 years of age (mean 24.3 years of age); 79.5% were <30 years of age. In total, 72 isolates were cultured from the urethra, 11 from urine, 3 from the cervix, 2 from the vagina (in children 4 and 6 years of age), 1 from the pharynx, and 7 from an unreported site.

The isolates were collected in 7/24 provinces. Among these, Córdoba and Ciudad Autónoma de Buenos Aires (CABA), 2 of the most populated provinces in Argentina, had the highest percentage of isolates (Córdoba had 47.9%; CABA had 39.6%) (Figure 1). We observed a lower percentage of isolates from the provinces of Buenos Aires (5.2%), Rio Negro (3.1%), Neuquén (2.1%), La Pampa (1.0%), and Santa Fe (1.0%).

Overall, 78 (81.3%) isolates had azithromycin MICs of 2–4 μg/mL, 13 (13.5%) had MICs of 8–16 μg/mL, and 5 (5.2%) had MICs of >256 μg/mL (Table 1). Among 5 isolates with MICs >256 μg/mL, 3 were collected in CABA in 2001 (n = 1) and 2019 (n = 2); the other 2 isolates were collected in Buenos Aires in 2018 and Córdoba in 2019. All 96 azithromycin-resistant isolates were susceptible to ceftriaxone, cefixime, and spectinomycin. However, 2 isolates collected in 2016 from Córdoba, each had a MIC of 4 μg/mL, showed decreased susceptibility to ceftriaxone (MIC = 0.06 μg/mL) and cefixime (MIC = 0.125 μg/mL) (Table 2).

All 5 isolates with MICs of >256 μg/mL had the A2059G mutation in all 4 23S rRNA alleles, whereas none of the 91 isolates with MICs of 2–16 μg/mL had this SNP (Table 1). Most (72; 75%) isolates with MICs of 2–16 μg/mL had the 23S rRNA C2611T mutation. Nearly all (70; 97.2%) of these isolates had the C2611T mutation in all 4 23S rRNA alleles, except for 2 isolates: 1 with a single mutated allele that had a MIC of 4 μg/mL and 1 with 3 mutated alleles that had a MIC of 8 μg/mL. Interspecies mosaics in the mtr locus (which encodes the tripartite MtrCDE efflux pump), as well as mutations in the mtrR promoter, coding region, or both, have been associated with increased azithromycin MICs (38–40). Among the 80 (83.3%) isolates with mtrR mutations, 17 (17.7%) had an mtrR-35A promoter deletion, 44 (45.8%) had an MtrR G45D amino acid mutation, 1 (1.0%) had an mtrR-35A deletion and MtrR G45D substitution, and 18 (18.8%) had a mosaic N. meningitidis–like mtrR promoter. We did not identify any isolates with the mtr₁₂₀ mutation. Eighteen isolates, all of which had MICs of 2–4 μg/mL, had no 23S rRNA mutations; however, 13 contained a mosaic mtrR promoter and 5 had a mtrR-35A deletion. Among 18 isolates with mosaic mtrR promoters, 100% also had mosaic sequences in the mtrD, 100% in mtrC, and 94.4% in mtrE loci. Fifteen isolates with a mosaic mtrD allele had sequences identical to the N. meningitidis–like mosaic previously described (39,40); 2 isolates had sequences sharing 97.8% identity and 1 had a sequence sharing 97.3% identity with the N. meningitidis–like mosaic (Appendix Figure 1). Isolates containing a mosaic-like mtr locus had MICs of >2 to >256 μg/mL. Isolates with MICs of >256 μg/mL also contained the 23S rRNA A2059G mutation.

We did not find any mutations associated with macrolide resistance in the rplD gene, which encodes ribosomal protein L4, or the rplV gene, which encodes ribosomal protein L22 (23). In addition, we did not find AMR mutations in macAB, which encodes the MacA-MacB efflux pump, or the acquired macrolide resistance genes, ere, mef, erm, mph, and msr (38). An isolate that had a MIC of 2 μg/mL had an unclear resistance mechanism.

Among the 96 N. gonorrhoeae isolates, we observed 42 NG-MAST STs, including 21 new STs and 25 STs represented by single isolates. We found 24 isolates belonging to ST470, 7 belonging to ST20102, 6 belonging to ST696, 4 belonging to ST12302, and 4 belonging to ST20104. We found 3 NG-MAST genogroups comprising >3 isolates: 33 belonged to G470, 10 belonged to G12302, and 10 belonged to G20102. We also documented 14 MLST STs, including 2 new STs and 8 STs represented by single isolates. We found 43 isolates belonging to ST1580, 14 belonging to ST1901, 14 belonging to ST9363, and 10 belonging to ST1584. NG-STAR showed 32 types, of which 11 were new and 20 were represented by single isolates. We found 32 isolates belonging to NG-STAR type 1038, 10 belonging to type 179, 5 belonging to type 168, and 5 belonging to type 3200.

Analysis of the phylogenomic tree revealed 14 clades. In total, 63 (65.6%) isolates were grouped into 3 clades, each containing 10–38 isolates (Figure 2) (https://microreact.org/project/AZM_Project/006b822d). The remaining 33 isolates were singletons or belonged to smaller clonal groups of 2–6 isolates each.

Clade 1 comprised 38 isolates, most of which belonged to NG-MAST G470 (86.8%), MLST ST1580 (97.4%), or NG-STAR ST1038 (84.2%). Clade 1 isolates had mean SNP difference of 8.5 (range 0–39). The isolates required MICs of 2–16 μg/mL; most (76.3%; 29/38) required an MIC of 4 μg/mL. The oldest isolate in clade 1 was identified in CABA in 2013. The proportion of clade 1 isolates increased significantly from 1.0% (1/96) in 2013 to 11.4% (11/96) in 2019 (p<0.05). Clade 1 was dominated by isolates from Córdoba (52.6%; 20/38) and CABA (28.9%; 11/38) but also included isolates obtained in 4 additional provinces. In total, 92.1% of the clade 1 isolates were from male patients and 7.9% were from female patients. Clade 1 isolates were characterized by the 23S rRNA C2611T mutation in all 4 alleles and the MtrR G45D amino acid mutation.

Clade 2 comprised 15 isolates that mainly belonged to NG-MAST G12302 (66.7%) and MLST ST9363 (93.3%). Clade 2 isolates had a mean SNP difference of 13.1 (range 0–33). All clade 2 isolates were cultured from men. Most (73.3%; 11/15) required an MIC of 2 μg/mL, and 26.7% (4/15) required MICs of >256 μg/mL. The first clade 2 isolate was detected in Córdoba in 2016; during 2017–2019, isolates were mainly detected in CABA (71.4%; 10/14), except for 2 isolates detected in Córdoba, 1 in Neuquén, and 1 in Buenos Aires. Clade 2 isolates did not have the 23S rRNA C2611T mutation but possessed the mosaic mtrR promoter and mtrCDE locus. In addition, isolates requiring MICs of >256 μg/mL had the 23S rRNA A2059G mutation in all 4 alleles.

Clade 3 was composed of 10 isolates belonging to NG-MAST G20102 and MLST ST1584. Clade 3 isolates had a mean SNP difference of 1.1 (range 0–2). Eight isolates were collected in Córdoba, 1 in CABA, and 1 in Río Negro during 2017–2019; of these, 8 were from men. All isolates required an MIC of 4 μg/mL and possessed the 23S rRNA C2611T mutation in all 4 alleles.

To investigate the international context of the 2 major MLST STs in Argentina, including azithromycin-resistant ST1580 and ST9363, we conducted a phylogenomic analysis using SNPs (Figure 3) (https://microreact.org/project/AZM_Project_2/7a2032e2). The ST1580 isolates from Argentina clustered with isolates from the United States, the United Kingdom (particularly Scotland), Australia, and Brazil. The mean pairwise SNP differences between ST1580 isolates from Argentina and other countries were 6.8 (range 1–23) for the isolates from the United States, 6.9 (range 1–22) for isolates from Australia, 7.9 (range 4–22) for isolates from Scotland, 11.4 (range 4–28) for isolates from Brazil, and 16.8 (range 13–31) for isolates from the United Kingdom (excluding Scotland). Isolates from Scotland and the United Kingdom had MICs of >256 μg/mL whereas isolates from the United States, Australia, and Brazil had MICs of 2–8 μg/mL. All isolates with MICs of 2–8 μg/mL had the 23S rRNA C2611T mutation and all isolates with MICs of >256 μg/mL had the A2059G mutation. In addition, 2 isolates from Brazil had mosaic mtrD alleles, but no mutations in the 23S rRNA gene; these isolates had MICs of 2 μg/mL. The ST9363 isolates from Argentina clustered with other ST9363 isolates from the United States, Australia, Canada, Brazil, and Norway. ST9363 isolates from Argentina had a mean pairwise SNP difference of 7.7 (range 0–20) with isolates from Brazil, 10.1 (range 1–23) with isolates from Norway, 12.5 (range 5–25) with isolates from Canada, 13.1 ( range 2–42) with isolates from the United States, and 14.8 (range 2–35) with isolates from Australia. All isolates had mosaic mtrR promoters and mtrD alleles. All isolates with MICs of >256 μg/mL had the 23S rRNA A2059G mutation and 4 isolates with MICs of 8–16 μg/mL had the 23S rRNA C2611T mutation.