ABSTRACT
Monitoring the emergence of antibiotic resistance is a recent issue in the treatment of Legionnaires' disease. Macrolides are recommended as first-line therapy, but resistance mechanisms have not been studied in Legionella species. Our aim was to determine the molecular basis of macrolide resistance in L. pneumophila. Twelve independent lineages from a common susceptible L. pneumophila ancestral strain were propagated under conditions of erythromycin or azithromycin pressure to produce high-level macrolide resistance. Whole-genome sequencing was performed on 12 selected clones, and we investigated mutations common to all lineages. We reconstructed the dynamics of mutation for each lineage and demonstrated their involvement in decreased susceptibility to macrolides. The resistant mutants were produced in a limited number of passages to obtain a 4,096-fold increase in erythromycin MICs. Mutations affected highly conserved 5-amino-acid regions of L4 and L22 ribosomal proteins and of domain V of 23S rRNA (G2057, A2058, A2059, and C2611 nucleotides). The early mechanisms mainly affected L4 and L22 proteins and induced a 32-fold increase in the MICs of the selector drug. Additional mutations related to 23S rRNA mostly occurred later and were responsible for a major increase of macrolide MICs, depending on the mutated nucleotide, the substitution, and the number of mutated genes among the three rrl copies. The major mechanisms of the decreased susceptibility to macrolides in L. pneumophila and their dynamics were determined. The results showed that macrolide resistance could be easily selected in L. pneumophila and warrant further investigations in both clinical and environmental settings.
KEYWORDS: 23S rRNA, Legionella pneumophila, macrolide, resistance, ribosomal mutations, ribosomal proteins
INTRODUCTION
Legionella, the causative agent of Legionnaires' disease (LD), is an intracellular Gram-negative bacterium of environmental origin. Among more than 70 species and serogroups, Legionella pneumophila serogroup 1 (Lp1) is involved in more than 85% of cases (1). Upon inhalation of contaminated aerosols from man-made or natural water systems, L. pneumophila can infect and replicate within lung macrophages. Treatments with antibiotics such as macrolides or fluoroquinolones that accumulate within these cells are effective therapies.
Following the first outbreak of LD that occurred in 1976 among American Legionnaires in Philadelphia, erythromycin was proposed as the drug of choice for the treatment of LD (2). Several years later, azithromycin and clarithromycin were found to be superior to erythromycin against intracellular L. pneumophila in vitro and in a guinea pig model (3–5).
The current American and European guidelines recommend macrolides as first-line therapy for the treatment of severe and moderate LD, with a preference for azithromycin (6, 7). However, treatment failures have been described and a mortality rate of over 10% is still reported in LD patients despite timely and adequate therapy (8, 9). No clinical or environmental macrolide-resistant strains have been isolated so far among Legionella species, and susceptibility testing is almost never performed on Legionella strains (10). However, the recent descriptions of emerging fluoroquinolone resistance in clinical settings may change this outlook (11, 12).
In vitro selection of erythromycin resistance in Legionella by one- or two-step procedures has ever been reported, but the molecular mechanisms have not been investigated so far (13, 14). We therefore characterized these mechanisms by investigation of independent L. pneumophila lineages from the same L. pneumophila ancestral strain propagated to high-level resistance by serial passages under conditions of increasing erythromycin or azithromycin concentrations. We identified mutations that occurred during the evolution procedure by whole-genome sequencing (WGS) performed on one clone from each macrolide-resistant evolved lineage and focused on the major determinants of the decreased susceptibility to macrolides, affecting genes encoding 23S rRNA (rrl), L4 (rplD), and L22 (rplV) ribosomal proteins in all lineages.
RESULTS
Selection of macrolide-resistant lineages of L. pneumophila.
The selection procedures resulted in high macrolide resistance levels whatever the drug used. A 4,096-fold minimal increase in MICs of the selector drug (from 0.25 to 1,024 mg/liter) was obtained in 9 to 11 passages for erythromycin-selected lineages and in 7 to 14 passages for 3 azithromycin-selected lineages; for the remaining 3 azithromycin-selected lineages, the increase in the MICs was limited to 256 mg/liter after 20 passages (Table 1).
TABLE 1.
L. pneumophila lineage | Passage | Erythromycin MIC (mg/liter) | Azithromycin MIC (mg/liter) | Mutation(s)a |
||
---|---|---|---|---|---|---|
rrl (no. of mutated copies/total no. of copies) (23S rRNA) | rplD (L4 protein) | rplV (L22 protein) | ||||
Ery1 | P2 | 1 | — | G66D | ND | |
P6 | 4 | G2057A (1/3)b | G66D | ND | ||
P7 | 16 | G2057A (3/3) | ND | ND | ||
P9 | 32 | G2057A (3/3) + A2058G (1/3) | ND | ND | ||
P10 | 512 | G2057A (3/3) + A2059C (3/3) | ND | ND | ||
P13 | 1,024 | G2057A (3/3) + A2059C (3/3) | G66D | — | ||
Ery2 | P1 | 0.5 | ND | Q62K | ND | |
P2 | 1 | — | Q62R + G64E | — | ||
P8 | 16 | C2611A (1/3)b | ND | ND | ||
P9 | 128 | C2611A (3/3) | ND | — | ||
P10 | 1,024 | C2611G (3/3) | ND | ND | ||
P12 | 1,024 | C2611G (3/3) | Q62R + G64E | — | ||
Ery3 | P1 | 0.5 | ND | G66A | ND | |
P7 | 256 | C2611T (2/3) | ND | ND | ||
P9 | 512 | C2611T (3/3) | ND | — | ||
P12 | 1,024 | C2611T (3/3) | G66A | — | ||
Ery4 | P1 | 0.5 | ND | K65N | — | |
P3 | 2 | ND | G66A | K90M | ||
P7 | 16 | A2058T (2/3) | G66A | ND | ||
P8 | 512 | A2058T (3/3) | G66A | ND | ||
P12 | 1,024 | A2058T (3/3) | G66A | K90M | ||
Ery5 | P1 | 0.5 | — | K63Qb | ND | |
P2 | 2 | G2057A (3/3) | — | ND | ||
P3 | 8 | G2057A (3/3) | G66S | ND | ||
P5 | 32 | G2057A (3/3) | G66A | ND | ||
P7 | 128 | G2057A (3/3) + A2059G (2/3) | G66A | ND | ||
P10 | 1,024 | G2057A (3/3) + A2058C (1/3) + A2059G (2/3)c | G66A | ND | ||
P12 | 1,024 | G2057A (3/3) + A2058C (2/3) + A2059G (1/3)c | G66A | — | ||
Ery6 | P3 | 1 | ND | G66D | ND | |
P4 | 2 | C2611A (2/3) | ND | ND | ||
P5 | 8 | C2611A (3/3) | ND | ND | ||
P8 | 64 | C2611A (1/3) + C2611T (2/3) | ND | — | ||
P10 | 1,024 | C2611T (3/3) | ND | ND | ||
P15 | 1,024 | C2611T (3/3) | G66D | — | ||
Azi1 | P3 | 1 | — | G66R | — | |
P4 | 1 | ND | T65K | ND | ||
P5 | 8 | — | T65K + G66R | ND | ||
P8 | 16 | C2611T (1/3)b | ND | ND | ||
P9 | 128 | C2611T (2/3)b | ND | ND | ||
P12 | 256 | C2611T (3/3) | ND | G91D | ||
P20 | 256 | C2611T (3/3) | T65K + G66R | G91D | ||
Azi2 | P4 | 128 | A2058G (2/3)b | — | — | |
P7 | 1,024 | A2058G (3/3) | ND | ND | ||
P10 | 2,048 | A2058G (3/3) | — | — | ||
Azi3 | P3 | 2 | — | T65K | ND | |
P7 | 32 | C2611T (3/3) | T65K | ND | ||
P9 | 64 | C2611T (3/3) | T65K + G66A | ND | ||
P12 | 128 | C2611T (3/3) | T65K + G66A | — | ||
P13 | 128 | ND | T65K + G66C | — | ||
P20 | 256 | C2611T (3/3) | T65K + G66C | — | ||
Azi4 | P3 | 1 | ND | del 63KG64 | ND | |
P8 | 8 | C2611G (2/3) | ND | ND | ||
P9 | 128 | C2611G (3/3) | del 63KG64 | ND | ||
P20 | 256 | C2611G (3/3) | del 63KG64 | — | ||
Azi5 | P2 | 2 | ND | T65K | — | |
P3 | 8 | ND | T65K | G91D | ||
P11 | 16 | — | ND | P87Lb + G91D | ||
P12 | 32 | A2058G (1/3)b | ND | ND | ||
P13 | 512 | A2058G (3/3) | ND | ND | ||
P16 | 1,024 | A2058G (3/3) | T65K | P87L + G91D | ||
Azi6 | P3 | 8 | C2611G (3/3) | ND | ND | |
P8 | 2,048 | A2058G (3/3) | — | — | ||
P12 | 2,048 | A2058G (3/3) | — | — |
E. coli numbering. —, no mutation; ND, not determined.
An additional subpopulation(s) was mutated.
Distinct rrl copies were mutated.
WGS data.
WGS data from the 12 clones showed that 4 to 14 mutations, involving 40 coding or noncoding sequences, occurred by lineage during the selection procedure. Mutations involving ribosomal rrl genes were common to all lineages. Other mutations notably affected genes encoding L4 and L22 ribosomal proteins (Table 1), putative efflux component proteins, a phosphate transporter, major outer membrane protein, conserved proteins of unknown function, and global transcriptional regulators.
Mutations in genes encoding 23S rRNA and L4 and L22 ribosomal proteins.
The observed mutations affected four nucleotides of domain V of 23S rRNA in the final clones. Nine mutations were detected: G2057A (Escherichia coli numbering), A2058T, A2058C, A2058G, A2059C, A2059G, C2611A, C2611G, and C2611T (Table 2). Specific PCRs performed for each rrl copy (n = 3) showed that at least two copies were mutated in each independent lineage. With the exception of Azi2 and Azi6, which had no mutation in genes encoding ribosomal proteins, all mutants showed one or several additional mutations in the rplD gene resulting in substitutions or deletions between the Q62 and G66 amino acids of the L4 protein. Only three mutants had substitutions in the rplV gene, leading to a P87L, K90M, or G91D substitution in the L22 protein. In most cases, the targeted resequencing (next-generation sequencing [NGS]) performed on the final populations revealed that the ribosomal mutations identified in the 12 evolved clones represented the main population of the sample. One exception was observed; in the Ery1 lineage, mutation A2059C observed in the rrl gene of the sequenced clone (Table 2) was identified in only 33% of the whole population, whereas a A2058G substitution occurred in 67% of this population.
TABLE 2.
L. pneumophila strain | Nucleotidic or amino acid change(s) |
MICa |
|||||||||||||
---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|
23S rRNAb (no. of mutated copies/total no. of copies) | L4 | L22 | ERY | AZI | CLR | SPI | LIN | PRI | TEL | LZ | LVX | CIP | RIF | DOX | |
Ery1 | G2057A (3/3) + A2059C (3/3) | G66D | — | 1,024 | 2,048 | 256 | 100,000 | 512 | 0.25 | >4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
Ery2 | C2611G (3/3) | Q62R + G64E | — | 1,024 | 128 | 128 | 6,250 | 64 | 0.25 | 4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
Ery3 | C2611T (3/3) | G66A | — | 1,024 | 32 | 256 | 6,250 | 32 | 0.25 | 1 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
Ery4 | A2058T (2/3) | G66A | K90M | 1,024 | 1,024 | 256 | 100,000 | >512 | 0.5 | >4 | 8 | 0.032 | 0.016 | 0.0005 | 2 |
Ery5 | G2057A (3/3) + A2058C (2/3) + A2059G (1/3) | G66A | — | 1,024 | 2,048 | >256 | 100,000 | 512 | 0.5 | >4 | 8 | 0.032 | 0.016 | 0.0005 | 2 |
Ery6 | C2611T (3/3) | G66D | — | 1,024 | 64 | 64 | 6,250 | 256 | 0.125 | 1 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
Azi1 | C2611T (3/3) | T65K + G66R | G91D | 1,024 | 256 | 256 | 25,000 | 64 | 1 | >4 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
Azi2 | A2058G (3/3) | — | — | 1,024 | 2,048 | 512 | 12,500 | 256 | 0.25 | 4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
Azi3 | C2611T (3/3) | T65K + G66C | — | 2,048 | 256 | 256 | 25,000 | 32 | 0.25 | 4 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
Azi4 | C2611G (3/3) | del 63KG64 | — | 2,048 | 256 | 512 | 25,000 | 64 | 1 | >4 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
Azi5 | A2058G (3/3) | T65K | P87L + G91D | 1,024 | 1,024 | 256 | 25,000 | >512 | 1 | >4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
Azi6 | A2058G (3/3) | — | — | 2,048 | 2,048 | 512 | 12,500 | >512 | 0.125 | >4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L1 | A2058G (3/3) | — | — | ≥1,024 | 1,024 | 256 | 12,500 | >512 | 0.125 | >4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L2 | A2058G (2/3) | — | — | ≥1,024 | 1,024 | 32 | 6,250 | >512 | 0.06 | >4 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L3 | G2057T (3/3) | — | — | 16 | 32 | 4 | 780 | 64 | 0.125 | 1 | 32 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L4 | C2611T (2/3) | — | — | 256 | 8 | 4 | 1,560 | 64 | 0.25 | 1 | 8 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L5 | C2611G (3/3) | — | — | 128 | 8 | 4 | 1,560 | 64 | 0.25 | 1 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
ΔdotA L6 | — | G66R | — | 8 | 4 | 0.063 | 1,560 | 64 | 0.25 | 0.25 | 16 | 0.032 | 0.016 | 0.001 | 2 |
ΔdotA L7 | — | G66A | — | 4 | 2 | 0.063 | 1,560 | 64 | 0.25 | 0.25 | 16 | 0.032 | 0.016 | 0.001 | 2 |
Paris WT | — | — | — | 0.25 | 0.25 | 0.063 | 390 | 64 | 0.125 | 0.125 | 16 | 0.032 | 0.016 | 0.0005 | 2 |
Paris ΔdotA | — | — | — | 0.25 | 0.25 | 0.063 | 390 | 64 | 0.125 | 0.125 | 16 | 0.032 | 0.016 | 0.001 | 2 |
All MIC data represent milligrams per liter, except the spiramycin data, which represent IU per milliliter. ERY, erythromycin; AZI, azithromycin; CLR, clarithromycin; SPI, spiramycin; LIN, lincomycin; PRI, pristinamycin; TEL, telithromycin; LZ, linezolid; LVX, levofloxacin; CIP, ciprofloxacin; RIF, rifampin; DOX, doxycycline.
E. coli numbering. —, no mutation.
Two macrolide resistance profiles.
Two distinct macrolide resistance profiles were observed. The first (lineages Ery1, Ery4, Ery5, Azi2, Azi5, and Azi6) corresponded to high-level resistance to both erythromycin and azithromycin (MICs, ≥1,024 mg/liter) and high-level cross-resistance to other macrolides (clarithromycin MIC, ≥256 mg/liter; spiramycin MIC, ≥25,000 IU/ml) and lincomycin (MIC, ≥256 mg/liter). The second (lineages Ery2, Ery3, Ery6, Azi1, Azi3, and Azi4) corresponded to high-level resistance to erythromycin (MIC, ≥1,024 mg/liter) but lower-level resistance to other macrolides (azithromycin MIC, 32 to 256 mg/liter; clarithromycin MIC, 64 to 256 mg/liter; spiramycin MIC, 6,250 to 25,000 IU/ml). The lincomycin MIC increased moderately (from 64 to a maximum of 256 mg/liter).
Irrespective of the resistance profile, the susceptibility to pristinamycin was poorly affected (MICs, 0.5 to 8 mg/liter), unlike the susceptibility to telithromycin (MICs, ≥1 mg/liter). No cross-resistance to other antibiotic families was observed, suggesting the presence of specific molecular mechanisms of macrolide resistance (Table 2).
Dynamics of substitution.
The dynamics of substitutions were determined by specific PCR and sequencing of rrl (n = 3), rplD, and rplV genes from the whole bacterial populations frozen at each passage. Mutations affecting L4 protein occurred at early steps, after one to three passages. They were responsible for decreased susceptibility to erythromycin or azithromycin, with a 2- to 8-fold increase in the MIC (0.5 to 2 mg/liter). Additional mutations in rplD or rplV genes were associated with another increase in erythromycin or azithromycin MICs (from 1 to 16 mg/liter). Mutations in rrl genes mainly occurred in steps that followed and were correlated to another decrease in susceptibility, with MICs increased to 2 to 2,048 mg/liter (Table 1). The Sanger sequencing revealed a genetic heterogeneity of resistant populations, which may explain the transitions in substitutions observed in several lineages.
Mutations affecting 23S rRNA.
The MICs varied according to the number of mutated rrl copies, the mutated nucleotide, and the nature of the substitution. Decreased susceptibility to erythromycin (MIC, ≤32 mg/liter) was observed when the mutation G2057A (Ery1 and Ery5) occurred. High-level resistance to erythromycin and azithromycin (MICs, ≥1,024 mg/liter) corresponding to the first resistance profile described above was observed when the A2058 substitution occurred (Ery4, Azi2, Azi5, and Azi6). Mutations of A2059 (Ery1 and Ery5) were combined with other rrl mutations; the lineages concerned showed a resistance level similar to that observed when mutations of A2058 occurred. Lineages harboring a C2611G or C2611T mutation (Ery2, Ery3, Ery6, Azi1, Azi3, and Azi4) had high-level resistance to erythromycin (MICs, 1,024 mg/liter) and various levels of decreased susceptibility to azithromycin (MICs, 8 to 256 mg/liter), described above as the second resistance profile. Lineages harboring a C2611A transition (Ery2 and Ery6) showed decreased susceptibility to erythromycin at a level that was lower than that observed with the C2611G and C2611T transitions. Except for the Ery5, Azi2, and Azi6 lineages, the rrl mutations were combined with rplD and/or rplV mutations, which prevented us from rigorously demonstrating the relationship between rrl mutations and phenotypes of macrolide susceptibility.
Reconstruction of resistance alleles in the macrolide-susceptible ancestral strain.
The rrl mutations A2058G, C2611T, and C2611G and the substitutions G66A and G66R in protein L4 were successfully introduced in ΔdotA mutant lineages by natural transformation (Table 2). We failed in our attempts to introduce G2057A and rplV substitutions. However, a spontaneous mutant grew on an agar plate containing erythromycin and revealed G2057T substitutions in the three rrl copies in the ΔdotA mutant L3 lineage. Decreased susceptibility to both erythromycin (MIC, ≤8 mg/liter) and azithromycin (MIC, ≤4 mg/liter) was observed when mutations involving the rplD gene were introduced. The G2057T transition in the rrl gene induced higher erythromycin and azithromycin MICs (MICs, ≤16 mg/liter and ≤32 mg/liter, respectively). High-level resistance to erythromycin (MIC, ≥128 mg/liter) but moderately decreased susceptibility to azithromycin (MIC, 8 mg/liter) was observed when C2611G and C2611T mutations were introduced. High-level resistance to both erythromycin and azithromycin (MICs, ≥1,024 mg/liter) and to all macrolides was observed after the A2058G transition.
DISCUSSION
In this study, we propagated 12 independent lineages of L. pneumophila from the same susceptible ancestral strain to a high level of macrolide resistance. The resistant mutants were obtained in a limited number of passages under pressure from erythromycin or azithromycin, two macrolides historically and currently recommended for the treatment of LD (2, 6, 7). The lineages were all highly resistant to erythromycin, with a 4,096-fold increase in MIC, and revealed cross-resistance to other macrolides, with two distinct resistance profiles differing by their levels of azithromycin susceptibility, suggesting two pathways toward high-level resistance. No cross-resistance to other families of antibiotics was observed, suggesting the presence of specific resistance mechanisms.
The characterization of the genetic events consisted first in a WGS strategy using a single evolved clone for each lineage that was representative of the whole population. We focused on mutations affecting L4 and L22 ribosomal proteins and 23S rRNA that were identified in all lineages and are involved in macrolide resistance in many other bacterial species (15, 16). The evolutionary pathway was determined for each lineage from frozen bacterial mixtures in which we observed mixed populations, stabilization of the resistance profiles, or, conversely, loss of the previously acquired mutations during the evolution procedure. In all lineages, additional steps led to a final high resistance level, without any prerequisite mutation necessary to achieve high-level resistance, unlike fluoroquinolone resistance in L. pneumophila (17). Most increases in macrolide MICs were correlated with additional mutations in the ribosomal targets. We also demonstrated the direct involvement of any mutations in macrolide susceptibility by reconstructing these mutations in the ancestral strain.
Point mutations or insertions/deletions in rplD or rplV genes occurred mainly in the early steps of the evolution procedure. They affected two highly conserved regions of 5 amino acids in L4 (Q62 to G66) and L22 (P87 to G91) proteins, which are located on loops that converge to form a narrowing structure in the ribosomal exit tunnel near the macrolide-binding site (18, 19). In E. coli, such mutations disrupt the conformation of residues in domains II, III, and V of 23S rRNA and result in a conformational change in the ribosome that hinders binding of macrolides to the peptide exit tunnel (20). In our study, these were associated with a moderate decrease in macrolide susceptibility, with a 2- to 64-fold increase in the MIC of the selector drug, and with moderate and inconsistent cross-resistance to other macrolides. They did not have an impact on lincomycin, pristinamycin, and telithromycin MICs.
Similar resistance levels have been described for other respiratory pathogens. Peric et al. showed that L4/L22 substitutions were responsible for a 2- to 32-fold increase in erythromycin and azithromycin MICs in Haemophilus influenzae clinical isolates (21). In Streptococcus pneumoniae, L4 and L22 alterations were responsible for a higher macrolide resistance level, with inconstant levels of cross-resistance to telithromycin but no impact on clindamycin MICs (22, 23). However, the susceptibility to the macrolide antibiotic family has been more widely studied using in vitro-selected mutants. As reported for L. pneumophila, a moderate increase in the macrolide MICs was observed for L4 and L22 mutants in in vitro-selected H. influenzae or Mycoplasma pneumoniae. Depending on the strain and the mutation, unmodified, increasing, or even decreasing clindamycin MICs have been described in H. influenzae mutants whereas telithromycin MICs were unaffected (24, 25). The cumulative effect of L4/L22 alterations observed in L. pneumophila was also described for these two species (21, 25). Unlike M. pneumoniae, they were not prerequisite for rrl mutations in L. pneumophila (25).
In L. pneumophila, as in M. pneumoniae, S. pneumoniae, Campylobacter jejuni, or Francisella tularensis, rrl mutations have been correlated to a higher resistance level, with selector drug MICs increased from 2 to 2,048 mg/liter (25–28). They were related to 4 nucleotides within the peptidyltransferase region (positions 2057, 2058, 2059, and 2611 in domain V of 23S rRNA), positions 2058 and 2059 being key nucleotides for macrolide binding and base pair 2057 and 2611 closing the stem preceding the single-stranded portion of the peptidyltransferase region (29).
The macrolide MICs of L. pneumophila varied first according to the number of mutated rrl copies, irrespective of the mutated nucleotide. Similar results have been described for positions 2057 in F. tularensis and 2059 in C. jejuni/C. coli, species that possess 3 copies of a ribosomal operon (28, 30). However, for positions 2058 and 2611, this contrasted with literature data: high-resistance level was reached as soon as one substitution occurred in a sole position 2058 nucleotide in F. tularensis, Ureaplasma parvum (2 copies), or S. pneumoniae (4 copies) and at position 2611 in S. pneumoniae (28, 31–33).
The macrolide MICs of the L. pneumophila mutants described here also varied widely according to the affected nucleotide. Although not all of the rrl mutations could be reconstructed, we confirmed a high- and cross-resistance profile for all macrolides when A2058 was mutated. Lower macrolide MICs, particularly those of 15- and 16-membered macrolides (azithromycin and spiramycin), were observed when mutations of G2057 or C2611 were introduced. Mutations involving G2057, observed in intermediate passages, were responsible for a moderate decrease in susceptibility for all macrolides. Our results did not allow any formal conclusion with respect to A2059 mutations, but the results observed with the Ery5 lineage let us hypothesize a resistance level similar to that seen with A2058 transitions. These observations correlate with literature data for many other bacterial species: mutations involving base 2058 or base 2059 are responsible for a high level of resistance to all macrolides. They usually give a higher advantage to the bacteria than substitutions in the base pair G2057 and C2611 (16, 25, 28, 31, 34–36).
The macrolide susceptibility of the L. pneumophila mutants described here also varied according to the nature of the substitution at C2611. C-to-T and -G transitions were responsible for higher MICs than the C-to-A transition, as observed in M. pneumoniae and S. pneumoniae (23, 32, 37). As also described for U. parvum and S. pneumoniae, the ribosomal mutations in L. pneumophila did not increase or increased only weakly the MICs of streptogramins, while ketolide MICs were affected, although their use is not recommended in clinical settings (26, 31).
A final point of note is that combinations of substitutions, such as mutations at positions 2058 and 2059 within a given rrl copy, were not observed, as described in many species, with the exception of C. jejuni (38). Furthermore, mutations in both the 2057–2059 region and position 2611 were not observed in L. pneumophila although they have been described in M. pneumoniae, C. jejuni, and S. pneumoniae. But this may have been due to the limited number of L. pneumophila lineages selected (23, 38, 39).
Resistance to macrolides can reduce the fitness of bacteria in the absence of antibiotics (40). To determine if the ribosomal macrolide resistance-conferring mutations observed in our study may or may not carry a biological cost, the bacterial fitness of the reconstructed resistant clones was studied. It was unaffected by the ribosomal mutations (data not shown). Bacterial fitness of the 12 sequenced clones was not studied as these strains possess second-site and nonribosomal mutations that might affect the function of conserved proteins and global transcriptional regulators and thus might positively interfere with their fitness.
Our experimental selection procedure did not allow any resistance mechanism involving horizontal gene transfer that might occur in Legionella-infected lungs (41). Mutations in rrl usually predominate in species with less than 4 operons, whereas 23S rRNA methylation is observed in species with more operons, such as staphylococci or streptococci, suggesting that the ribosomal mutations described here might be the major macrolide resistance mechanism in Legionella species in vivo (16). Macrolides are the first-line antibiotics for LD therapy (6, 7). Treatment failures have been reported, suggesting the possibility of resistance acquired in vivo (8, 9). Yet no macrolide-resistant clinical strain has been isolated so far. Legionella are consistently susceptible to macrolide antibiotics in axenic medium and in cell or animal models (3–5, 42, 43). These data contrast with the ease with which strains with high-level resistance were selected in vitro in our study.
Antimicrobial susceptibility testing is not routinely performed on Legionella strains, even in expert laboratories, except in cases in which the patient is critically ill or relapsing. Isolation of Legionella strains remains difficult, and a preceding antibiotic therapy can cause a negative culture result despite persistence of the infection (44, 45). Moreover, Legionella is an environmental pathogen for which humans are accidental hosts. With one exception, no human-to-human spread has been reported so far (46). Unlike respiratory pathogens such as Staphylococcus aureus or Mycobacterium tuberculosis, for which antibiotic resistance is a major issue, Legionella strains that would acquire mutations under macrolide therapy would not be infectious for other hosts. Combination therapy is advocated to treat severe LD, but there is no evidence of its superiority over monotherapy (47–50). Moffie and Mouton described a mutation rate of 10−7 for erythromycin, while the Legionella burden in lower respiratory tract samples ranges from 2 to 8 log10 DNA copies/ml according to LD severity (51, 52). Thus, the use of combination therapy for critically ill patients may also contribute to limiting the emergence of macrolide-resistant Legionella strains. Taking the data together, the combination of a low rate of isolation from clinical samples, the limitation of susceptibility testing to severely ill patients, the absence of human-to-human spread, and the use of combined therapy for patients with high bacterial burden probably help to explain why no macrolide-resistant clinical isolate has been reported so far. In this study, we demonstrated that high-level macrolide-resistant mutants can be easily and quickly selected in vitro. Such in vivo selection should be considered and may constitute an argument warranting systematic antibiotic combinations for severe LD and for immunosuppressed patients.
Alternatively to mutations occurring under therapy, patients could contract a Legionella-resistant strain directly from the environment. Macrolides are present in natural environments, as they are produced by Streptomycetes species. They are mostly and extensively used in human and veterinary medicines (notably aquaculture) to control and treat infectious diseases. Administered at subtherapeutic doses, they also act as growth promoters in livestock in veterinary medicine (53). Macrolide antibiotics have been detected in treated wastewater effluents (the main source being hospital and aquaculture effluents) and in river waters but also in surface water, groundwater, and drinking water in a range of nanograms per liter to micrograms per liter, which highlights the direct exposure of Legionella to macrolide drugs in its natural habitat (54). The diffusion of macrolides in the environment, particularly in natural water systems, contributes to the development of antibiotic resistance that may affect Legionella species (55).
In conclusion, we found that L. pneumophila mutants with high-level resistance could be easily selected in vitro by the use of subinhibitory concentrations of macrolides. Although they were not prerequisite, initial mechanisms mainly involved ribosomal L4/L22 proteins and induced moderated decreased susceptibility to macrolides. Additional mutations in genes encoding 23S rRNA mostly occurred in a second step and were responsible for a major increase of the resistance level. The data warrant further investigations in both clinical and environmental settings and promote the development of PCR assays targeting the mutated Legionella rrl genes and/or deep-sequencing approaches, which might be notably implemented on culture-negative samples.
MATERIALS AND METHODS
Bacterial strains and culture media.
The reference strain L. pneumophila serogroup 1 (Lp1) Paris (CIP 107629T) was used to select macrolide-resistant strains. Bacteria were grown in N-(2-acetamido)-2-aminoethanesulfonic acid (ACES)-buffered yeast extract (BYE) broth at 37°C in an aerobic atmosphere or on buffered-charcoal-yeast extract (BCYE) agar plates (Oxoid, Dardilly, France) at 35°C in a 2.5% CO2-enriched atmosphere.
The avirulent strain Lp1 Paris, deleted for dotA by a unique insertion of a kanamycin cassette (dotA::kan), was used to select macrolide-resistant strains by natural transformation (56, 57).
Antibiotics.
The following antimicrobial agents were tested: erythromycin, azithromycin, clarithromycin, rifampin, doxycycline (Sigma-Aldrich, Saint-Quentin-Fallavier, France), spiramycin, pristinamycin, telithromycin, levofloxacin (Sanofi, Gentilly, France), lincomycin, linezolid (Pfizer, Amboise, France), and ciprofloxacin (Bayer, Puteaux, France). Antibiotic solutions were prepared at 64 mg/ml and stored at −20°C until use.
Selection of macrolide-resistant mutants of L. pneumophila.
Selection of six independent erythromycin-resistant lineages (namely, Ery1 to Ery6) and six independent azithromycin-resistant lineages (Azi1 to Azi6) was performed in a biosafety level 3 laboratory by serial passages in BYE medium containing increasing subinhibitory concentrations of erythromycin and azithromycin, respectively. A suspension of the Lp1 Paris strain (final concentration, 4.105 CFU/ml) in BYE broth was dispensed in 24-well microtiter plates (BD Falcon; Becton Dickinson, Le Pont-de-Claix, France) containing erythromycin or azithromycin at increasing 2-fold concentrations ranging from a 0.5- to 16-fold change from the MIC determined for the ancestral strain. The plates were incubated for 3 to 4 days in an aerobic atmosphere at 35°C. The MIC was determined as the lowest antibiotic concentration that inhibited visible bacterial growth. The culture well containing the highest concentration of antibiotics with bacterial growth was used to propagate the lineages. After a 1:100 dilution, a subsequent passage was performed into new 24-well microtiter plates containing fresh medium, with increasing 2-fold concentrations ranging from a 0.5- to 16-fold change from the MIC previously determined. This procedure was repeated until growth was obtained at an erythromycin (Ery1 to Ery6) or azithromycin (Azi1 to Azi6) concentration of 1,024 mg/liter, corresponding to a 4,096-fold increase in the antibiotic MIC for the ancestral strain, or after 20 passages. At each evolution step, the contents of each well (genetically heterogeneous mixtures) were frozen at −80°C. Two additional consecutive passages were performed in a 0.5-fold MIC medium to assess the stability of the resistance phenotype before stopping the evolution procedure. The 12 final bacterial mixtures were sampled and frozen. One evolved clone per lineage was randomly selected for WGS on the basis of the assumption that it would be representative of the whole population.
WGS.
Genomes of the 12 evolved clones and the ancestral strain were sequenced using single-read 50-bp Illumina technologies at the ProfileXpert facility (Lyon, France). Reads were mapped against the reference genome (NC_006368). Mapping and variant calling were performed using CASAVA 1.8.2 software.
Dynamics of mutation.
The proportion of the population carrying the mutations in rrl, rplD, and rplV identified in the sequenced clone was first determined in the 12 final bacterial mixtures by performing specific PCR targeting the mutated regions and sequencing the amplicons by next-generation sequencing (NGS) technology. The amplifications were performed using Phusion High-Fidelity DNA polymerase (New England BioLabs, Evry, France). The amplicon libraries were generated using an Ion Plus Fragment library kit and were sequenced on an Ion Torrent PGM (Life Technologies, Saint Aubin, France) according to the manufacturer's instructions. Reads were mapped against the reference sequences extracted from the genome (NC_006368). Mapping and variant calling were performed using Torrent Suite 5.0.2.
The dynamics of mutation was determined retrospectively from the frozen intermediate bacterial mixtures by specific PCRs for each lineage (Table 3). The same primers were used for both amplification and sequencing, except for the 23S rRNA gene, for which specific primers were used to amplify independently the 3 copies of the gene and other primers were used to sequence the regions in which there were mutations. Briefly, all PCRs were performed using Expand High FidelityPLUS Taq polymerase (Roche Diagnostics, Meylan, France) and were carried out in 50-μl volumes containing a 0.4 μM concentration of each primer, 1 μl of DNA for the rrl PCR, and 10 μl of DNA for the rplD and rplV PCRs. Double-strand DNA sequencing was performed at the Biofidal facility (Vaulx-en-Velin, France).
TABLE 3.
Gene | Primer name | Primer sequence | Product size (bp) | PCR conditions |
|
---|---|---|---|---|---|
MgCl2 concn (mM) | Amplification conditions | ||||
rrla (copies no. 1, 2, and 3) | F2 | 5′-AAGGCATAGACAGCCAGGAG-3′ | |||
rrla (copy no. 1) | R1.3 | 5′-GCTTGCTAACTCACACCAAC-3′ | 2,573 | 1.5 | 1 cycle of 5 min at 95°C; 35 cycles of 15 s at 94°C, 30 s at 62°C, and 150 s at 72°C; 1 cycle of 5 min at 72°C |
rrla (copy no. 2) | R2''.2 | 5′-CAAGGAATCACGGTAGG-3′ | 2,566 | 1.5 | 1 cycle of 5 min at 95°C; 35 cycles of 15 s at 94°C, 30 s at 55°C, and 150 s at 72°C; 1 cycle of 5 min at 72°C |
rrla (copy no. 3) | R3.2 | 5′-GAACCAACAAGCATTCTC-3′ | 2,274 | 1.5 | 1 cycle of 5 min at 95°C; 35 cycles of 15 s at 94°C, 30 s at 55°C, and 150 s at 72°C; 1 cycle of 5 min at 72°C |
rrlb (copies no. 1, 2, and 3) | 23S F | 5′-AAGTTCCGACCTGCACGAAT-3′ | 859 | ||
23S R | 5′-GTAGTCTTCAACGGGCTTCA-3′ | ||||
rplDa,b | L4_F | 5′-AAAGGTGCAATTCCTGGTG-3′ | 897 | 3 | 1 cycle of 5 min at 95°C; 35 cycles of 15 s at 94°C, 35 s at 50°C, and 50 s at 72°C; 1 cycle of 5 min at 72°C |
L4_R | 5′-CTGGTTTGTTTGAAGCGTTTAG-3′ | ||||
rplVa,b | L22_F | 5′-GCATAACGCAAAGACCAC-3′ | 834 | 3 | 1 cycle of 5 min at 95°C; 35 cycles of 15 s at 94°C, 35 s at 50°C, and 50 s at 72°C; 1 cycle of 5 min at 72°C |
L22_R | 5′-AGCAATACCTTCAGCCACCA-3′ | ||||
rrlc (copies no. 1, 2, and 3) | F1 | 5′-GGAAAGTTGGCCGTAGAGG-3′ | |||
rrlc (copy no. 1) | R1.2 | 5′-TCCTTCGCCATCGGAAAGTC-3′ | 3,440 | 1.5 | 1 cycle of 1 min at 98°C; 35 cycles of 15 s at 98°C, 30 s at 58°C, and 120 s at 72°C; 1 cycle of 8 min at 72°C |
rrlc (copy no. 2) | R2.2 | 5′-AGGGCAAGGAATCACGGTAG-3′ | 3,302 | 1.5 | 1 cycle of 1 min at 98°C; 35 cycles of 15 s at 98°C, 30 s at 58°C, and 120 s at 72°C; 1 cycle of 8 min at 72°C |
rrlc (copy no. 3) | R3.5 | 5′-AGTGTTCTGCAAGTGGACAACTC-3′ | 3,505 | 1.5 | 1 cycle of 1 min at 98°C; 35 cycles of 15 s at 98°C, 30 s at 58°C, and 120 s at 72°C; 1 cycle of 8 min at 72°C |
rplDc | L4_MF | 5′-CAGCAGCTATTACAACGA-3′ | 4,855 | 3 | 1 cycle of 1 min at 98°C; 35 cycles of 15 s at 98°C, 30 s at 58°C, and 150 s at 72°C; 1 cycle of 8 min at 72°C |
L22_R | 5′-AGCAATACCTTCAGCCACCA-3′ | ||||
rplVc | L22_MF | 5′-CACGAGGTGAGTGATGGA-3′ | 4,674 | 3 | 1 cycle of 1 min at 98°C; 35 cycles of 15 s at 98°C, 30 s at 58°C, and 150 s at 72°C; 1 cycle of 8 min at 72°C |
L22_MR | 5′-AACACCATTACTCTCAAGA-3′ |
Primers used for DNA amplification.
Primers used for DNA sequencing (dynamics of substitutions).
Primers used for natural transformation.
Reconstruction of ribosomal mutations in the ancestral strain.
To confirm the involvement of rrl, rplD, and rplV mutations in the decreased susceptibility to macrolides, mutation reconstruction was performed by inducing competence for natural transformation in ΔdotA L. pneumophila strains in a biosafety level-2 laboratory, as previously described (56). PCR assays were performed using Phusion High-Fidelity DNA polymerase and specific primers (Table 3). Following natural transformation, the bacterial mixtures were plated on BCYE agar plates containing 50 mg/liter erythromycin (approximate final concentration after charcoal absorption, 5 mg/liter [58]) incubated in an aerobic atmosphere at 35°C and examined over 14 days. The presence of mutations in growing colonies was investigated by PCR amplification and sequencing.
Determination of MICs.
For each L. pneumophila clone to be tested, the MICs of antibiotics were determined in duplicate by a broth microdilution method previously described (59).
Accession number(s).
WG sequences were deposited in the European Nucleotide Archive (ENA) under BioProject accession number PRJEB14949.
ACKNOWLEDGMENTS
We thank Philip Robinson (DRCI, Hospices Civils de Lyon, France) for help in manuscript preparation.
We declare that we have no conflicts of interest.
REFERENCES
- 1.Carratalà J, Garcia-Vidal C. 2010. An update on Legionella. Curr Opin Infect Dis 23:152–157. doi: 10.1097/QCO.0b013e328336835b. [DOI] [PubMed] [Google Scholar]
- 2.Fraser DW, Wachsmuth IK, Bopp C, Tsai TF, Feeley JC. 1978. Antibiotics for legionnaires' disease. Lancet i:1045. [DOI] [PubMed] [Google Scholar]
- 3.Stout JE, Arnold B, Yu VL. 1998. Activity of azithromycin, clarithromycin, roxithromycin, dirithromycin, quinupristin/dalfopristin and erythromycin against Legionella species by intracellular susceptibility testing in HL-60 cells. J Antimicrob Chemother 41:289–291. doi: 10.1093/jac/41.2.289. [DOI] [PubMed] [Google Scholar]
- 4.Fitzgeorge RB, Lever S, Baskerville A. 1993. A comparison of the efficacy of azithromycin and clarithromycin in oral therapy of experimental airborne Legionnaires' disease. J Antimicrob Chemother 31(Suppl E):171–176. [DOI] [PubMed] [Google Scholar]
- 5.Fitzgeorge RB, Featherstone AS, Baskerville A. 1990. Efficacy of azithromycin in the treatment of guinea pigs infected with Legionella pneumophila by aerosol. J Antimicrob Chemother 25(Suppl A):101–108. [DOI] [PubMed] [Google Scholar]
- 6.Mandell LA, Wunderink RG, Anzueto A, Bartlett JG, Campbell GD, Dean NC, Dowell SF, File TM Jr, Musher DM, Niederman MS, Torres A, Whitney CG. 2007. Infectious Diseases Society of America/American Thoracic Society consensus guidelines on the management of community-acquired pneumonia in adults. Clin Infect Dis 44(Suppl 2):S27–S72. doi: 10.1086/511159. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 7.Woodhead M, Blasi F, Ewig S, Garau J, Huchon G, Ieven M, Ortqvist A, Schaberg T, Torres A, van der Heijden G, Read R, Verheij TJ. 2011. Guidelines for the management of adult lower respiratory tract infections. Clin Microbiol Infect 17(Suppl 6):E1–E59. doi: 10.1111/j.1469-0691.2011.03672.x. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 8.Tan JS, File TM Jr, DiPersio JR, DiPersio LP, Hamor R, Saravolatz LD, Stout JE. 2001. Persistently positive culture results in a patient with community-acquired pneumonia due to Legionella pneumophila. Clin Infect Dis 32:1562–1566. doi: 10.1086/320526. [DOI] [PubMed] [Google Scholar]
- 9.Gläser S, Weitzel T, Schiller R, Suttorp N, Lück PC. 2005. Persistent culture-positive Legionella infection in an immunocompetent adult. Clin Infect Dis 41:765–766. doi: 10.1086/432627. [DOI] [PubMed] [Google Scholar]
- 10.Onody C, Matsiota-Bernard P, Nauciel C. 1997. Lack of resistance to erythromycin, rifampicin and ciprofloxacin in 98 clinical isolates of Legionella pneumophila. J Antimicrob Chemother 39:815–816. doi: 10.1093/jac/39.6.815. [DOI] [PubMed] [Google Scholar]
- 11.Bruin JP, Koshkolda T, Ijzerman EP, Lück C, Diederen BM, Den Boer JW, Mouton JW. 2014. Isolation of ciprofloxacin-resistant Legionella pneumophila in a patient with severe pneumonia. J Antimicrob Chemother 69:2869–2871. doi: 10.1093/jac/dku196. [DOI] [PubMed] [Google Scholar]
- 12.Shadoud L, Almahmoud I, Jarraud S, Etienne J, Larrat S, Schwebel C, Timsit JF, Schneider D, Maurin M. 2015. Hidden selection of bacterial resistance to fluoroquinolones in vivo: the case of Legionella pneumophila and humans. EBioMedicine 2:1179–1185. doi: 10.1016/j.ebiom.2015.07.018. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 13.Dowling JN, McDevitt DA, Pasculle AW. 1985. Isolation and preliminary characterization of erythromycin-resistant variants of Legionella micdadei and Legionella pneumophila. Antimicrob Agents Chemother 27:272–274. doi: 10.1128/AAC.27.2.272. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 14.Nielsen K, Bangsborg JM, Hoiby N. 2000. Susceptibility of Legionella species to five antibiotics and development of resistance by exposure to erythromycin, ciprofloxacin, and rifampicin. Diagn Microbiol Infect Dis 36:43–48. doi: 10.1016/S0732-8893(99)00095-4. [DOI] [PubMed] [Google Scholar]
- 15.Diner EJ, Hayes CS. 2009. Recombineering reveals a diverse collection of ribosomal proteins L4 and L22 that confer resistance to macrolide antibiotics. J Mol Biol 386:300–315. doi: 10.1016/j.jmb.2008.12.064. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 16.Vester B, Douthwaite S. 2001. Macrolide resistance conferred by base substitutions in 23S rRNA. Antimicrob Agents Chemother 45:1–12. doi: 10.1128/AAC.45.1.1-12.2001. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 17.Almahmoud I, Kay E, Schneider D, Maurin M. 2009. Mutational paths towards increased fluoroquinolone resistance in Legionella pneumophila. J Antimicrob Chemother 64:284–293. doi: 10.1093/jac/dkp173. [DOI] [PubMed] [Google Scholar]
- 18.Mankin AS. 2008. Macrolide myths. Curr Opin Microbiol 11:414–421. doi: 10.1016/j.mib.2008.08.003. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 19.Nissen P, Hansen J, Ban N, Moore PB, Steitz TA. 2000. The structural basis of ribosome activity in peptide bond synthesis. Science 289:920–930. doi: 10.1126/science.289.5481.920. [DOI] [PubMed] [Google Scholar]
- 20.Gregory ST, Dahlberg AE. 1999. Erythromycin resistance mutations in ribosomal proteins L22 and L4 perturb the higher order structure of 23 S ribosomal RNA. J Mol Biol 289:827–834. doi: 10.1006/jmbi.1999.2839. [DOI] [PubMed] [Google Scholar]
- 21.Peric M, Bozdogan B, Jacobs MR, Appelbaum PC. 2003. Effects of an efflux mechanism and ribosomal mutations on macrolide susceptibility of Haemophilus influenzae clinical isolates. Antimicrob Agents Chemother 47:1017–1022. doi: 10.1128/AAC.47.3.1017-1022.2003. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 22.Tait-Kamradt A, Davies T, Appelbaum PC, Depardieu F, Courvalin P, Petitpas J, Wondrack L, Walker A, Jacobs MR, Sutcliffe J. 2000. Two new mechanisms of macrolide resistance in clinical strains of Streptococcus pneumoniae from Eastern Europe and North America. Antimicrob Agents Chemother 44:3395–3401. doi: 10.1128/AAC.44.12.3395-3401.2000. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 23.Farrell DJ, Morrissey I, Bakker S, Buckridge S, Felmingham D. 2004. In vitro activities of telithromycin, linezolid, and quinupristin-dalfopristin against Streptococcus pneumoniae with macrolide resistance due to ribosomal mutations. Antimicrob Agents Chemother 48:3169–3171. doi: 10.1128/AAC.48.8.3169-3171.2004. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 24.Clark C, Bozdogan B, Peric M, Dewasse B, Jacobs MR, Appelbaum PC. 2002. In vitro selection of resistance in Haemophilus influenzae by amoxicillin-clavulanate, cefpodoxime, cefprozil, azithromycin, and clarithromycin. Antimicrob Agents Chemother 46:2956–2962. doi: 10.1128/AAC.46.9.2956-2962.2002. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 25.Pereyre S, Guyot C, Renaudin H, Charron A, Bebear C, Bebear CM. 2004. In vitro selection and characterization of resistance to macrolides and related antibiotics in Mycoplasma pneumoniae. Antimicrob Agents Chemother 48:460–465. doi: 10.1128/AAC.48.2.460-465.2004. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 26.Canu A, Malbruny B, Coquemont M, Davies TA, Appelbaum PC, Leclercq R. 2002. Diversity of ribosomal mutations conferring resistance to macrolides, clindamycin, streptogramin, and telithromycin in Streptococcus pneumoniae. Antimicrob Agents Chemother 46:125–131. doi: 10.1128/AAC.46.1.125-131.2002. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 27.Caldwell DB, Wang Y, Lin J. 2008. Development, stability, and molecular mechanisms of macrolide resistance in Campylobacter jejuni. Antimicrob Agents Chemother 52:3947–3954. doi: 10.1128/AAC.00450-08. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 28.Gestin B, Valade E, Thibault F, Schneider D, Maurin M. 2010. Phenotypic and genetic characterization of macrolide resistance in Francisella tularensis subsp. holarctica biovar I. J Antimicrob Chemother 65:2359–2367. doi: 10.1093/jac/dkq315. [DOI] [PubMed] [Google Scholar]
- 29.Schlünzen F, Zarivach R, Harms J, Bashan A, Tocilj A, Albrecht R, Yonath A, Franceschi F. 2001. Structural basis for the interaction of antibiotics with the peptidyl transferase centre in eubacteria. Nature 413:814–821. doi: 10.1038/35101544. [DOI] [PubMed] [Google Scholar]
- 30.Ladely SR, Meinersmann RJ, Englen MD, Fedorka-Cray PJ, Harrison MA. 2009. 23S rRNA gene mutations contributing to macrolide resistance in Campylobacter jejuni and Campylobacter coli. Foodborne Pathog Dis 6:91–98. doi: 10.1089/fpd.2008.0098. [DOI] [PubMed] [Google Scholar]
- 31.Pereyre S, Metifiot M, Cazanave C, Renaudin H, Charron A, Bebear C, Bebear CM. 2007. Characterisation of in vitro-selected mutants of Ureaplasma parvum resistant to macrolides and related antibiotics. Int J Antimicrob Agents 29:207–211. doi: 10.1016/j.ijantimicag.2006.09.008. [DOI] [PubMed] [Google Scholar]
- 32.Tait-Kamradt A, Davies T, Cronan M, Jacobs MR, Appelbaum PC, Sutcliffe J. 2000. Mutations in 23S rRNA and ribosomal protein L4 account for resistance in pneumococcal strains selected in vitro by macrolide passage. Antimicrob Agents Chemother 44:2118–2125. doi: 10.1128/AAC.44.8.2118-2125.2000. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 33.Davies TA, Bush K, Sahm D, Evangelista A. 2005. Predominance of 23S rRNA mutants among non-erm, non-mef macrolide-resistant clinical isolates of Streptococcus pneumoniae collected in the United States in 1999–2000. Antimicrob Agents Chemother 49:3031–3033. doi: 10.1128/AAC.49.7.3031-3033.2005. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 34.Chisholm SA, Dave J, Ison CA. 2010. High-level azithromycin resistance occurs in Neisseria gonorrhoeae as a result of a single point mutation in the 23S rRNA genes. Antimicrob Agents Chemother 54:3812–3816. doi: 10.1128/AAC.00309-10. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 35.Rimbara E, Noguchi N, Kawai T, Sasatsu M. 2008. Novel mutation in 23S rRNA that confers low-level resistance to clarithromycin in Helicobacter pylori. Antimicrob Agents Chemother 52:3465–3466. doi: 10.1128/AAC.00445-08. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 36.Ross JI, Eady EA, Cove JH, Jones CE, Ratyal AH, Miller YW, Vyakrnam S, Cunliffe WJ. 1997. Clinical resistance to erythromycin and clindamycin in cutaneous propionibacteria isolated from acne patients is associated with mutations in 23S rRNA. Antimicrob Agents Chemother 41:1162–1165. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 37.Bébéar C, Pereyre S, Peuchant O. 2011. Mycoplasma pneumoniae: susceptibility and resistance to antibiotics. Future Microbiol 6:423–431. doi: 10.2217/fmb.11.18. [DOI] [PubMed] [Google Scholar]
- 38.Vacher S, Menard A, Bernard E, Santos A, Megraud F. 2005. Detection of mutations associated with macrolide resistance in thermophilic Campylobacter spp. by real-time PCR. Microb Drug Resist 11:40–47. doi: 10.1089/mdr.2005.11.40. [DOI] [PubMed] [Google Scholar]
- 39.Matsuoka M, Narita M, Okazaki N, Ohya H, Yamazaki T, Ouchi K, Suzuki I, Andoh T, Kenri T, Sasaki Y, Horino A, Shintani M, Arakawa Y, Sasaki T. 2004. Characterization and molecular analysis of macrolide-resistant Mycoplasma pneumoniae clinical isolates obtained in Japan. Antimicrob Agents Chemother 48:4624–4630. doi: 10.1128/AAC.48.12.4624-4630.2004. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 40.Melnyk AH, Wong A, Kassen R. 2015. The fitness costs of antibiotic resistance mutations. Evol Appl 8:273–283. doi: 10.1111/eva.12196. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 41.Roberts MC. 2008. Update on macrolide-lincosamide-streptogramin, ketolide, and oxazolidinone resistance genes. FEMS Microbiol Lett 282:147–159. doi: 10.1111/j.1574-6968.2008.01145.x. [DOI] [PubMed] [Google Scholar]
- 42.Schrock J, Hackman BA, Plouffe JF. 1997. Susceptibility of ninety-eight clinical isolates of Legionella to macrolides and quinolones using the Etest. Diagn Microbiol Infect Dis 28:221–223. doi: 10.1016/S0732-8893(97)00043-6. [DOI] [PubMed] [Google Scholar]
- 43.Pendland SL, Martin SJ, Chen C, Schreckenberger PC, Danziger LH. 1997. Comparison of charcoal- and starch-based media for testing susceptibilities of Legionella species to macrolides, azalides, and fluoroquinolones. J Clin Microbiol 35:3004–3006. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 44.Schindel C, Siepmann U, Han S, Ullmann AJ, Mayer E, Fischer T, Maeurer M. 2000. Persistent Legionella infection in a patient after bone marrow transplantation. J Clin Microbiol 38:4294–4295. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 45.Descours G, Tellini C, Flamens C, Philit F, Celard M, Etienne J, Lina G, Jarraud S. 2013. Legionellosis and lung abscesses: contribution of Legionella quantitative real-time PCR to an adapted followup. Case Rep Infect Dis 2013:190183. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 46.Borges V, Nunes A, Sampaio DA, Vieira L, Machado J, Simoes MJ, Goncalves P, Gomes JP. 2016. Legionella pneumophila strain associated with the first evidence of person-to-person transmission of Legionnaires' disease: a unique mosaic genetic backbone. Sci Rep 6:26261. doi: 10.1038/srep26261. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 47.Rello J, Gattarello S, Souto J, Sole-Violan J, Valles J, Peredo R, Zaragoza R, Vidaur L, Parra A, Roig J; Community-Acquired Pneumonia in Unidad de Cuidados Intensivos 2 CAPUCI 2 Study Investigators. 2013. Community-acquired Legionella pneumonia in the intensive care unit: impact on survival of combined antibiotic therapy. Med Intensiva 37:320–326. doi: 10.1016/j.medin.2012.05.010. [DOI] [PubMed] [Google Scholar]
- 48.Nakamura S, Yanagihara K, Izumikawa K, Seki M, Kakeya H, Yamamoto Y, Senjyu H, Saito A, Kohno S. 2009. The clinical efficacy of fluoroquinolone and macrolide combination therapy compared with single-agent therapy against community-acquired pneumonia caused by Legionella pneumophila. J Infect 59:222–224. doi: 10.1016/j.jinf.2009.06.008. [DOI] [PubMed] [Google Scholar]
- 49.Grau S, Antonio JM, Ribes E, Salvado M, Garces JM, Garau J. 2006. Impact of rifampicin addition to clarithromycin in Legionella pneumophila pneumonia. Int J Antimicrob Agents 28:249–252. doi: 10.1016/j.ijantimicag.2006.03.029. [DOI] [PubMed] [Google Scholar]
- 50.Benito JR, Montejo JM, Cancelo L, Zalacain R, Lopez L, Fernandez Gil de Pareja J, Alonso E, Onate J. 2003. Community-acquired pneumonia due to Legionella pneumophila serogroup 1. Study of 97 cases. Enferm Infecc Microbiol Clin 21:394–400. (In Spanish.) [PubMed] [Google Scholar]
- 51.Moffie BG, Mouton RP. 1988. Sensitivity and resistance of Legionella pneumophila to some antibiotics and combinations of antibiotics. J Antimicrob Chemother 22:457–462. doi: 10.1093/jac/22.4.457. [DOI] [PubMed] [Google Scholar]
- 52.Maurin M, Hammer L, Gestin B, Timsit JF, Rogeaux O, Delavena F, Tous J, Epaulard O, Brion JP, Croize J. 2010. Quantitative real-time PCR tests for diagnostic and prognostic purposes in cases of legionellosis. Clin Microbiol Infect 16:379–384. doi: 10.1111/j.1469-0691.2009.02812.x. [DOI] [PubMed] [Google Scholar]
- 53.Carvalho IT, Santos L. 2016. Antibiotics in the aquatic environments: a review of the European scenario. Environ Int 94:736–757. doi: 10.1016/j.envint.2016.06.025. [DOI] [PubMed] [Google Scholar]
- 54.Kümmerer K. 2009. Antibiotics in the aquatic environment–a review–part I. Chemosphere 75:417–434. doi: 10.1016/j.chemosphere.2008.11.086. [DOI] [PubMed] [Google Scholar]
- 55.Xu J, Xu Y, Wang H, Guo C, Qiu H, He Y, Zhang Y, Li X, Meng W. 2015. Occurrence of antibiotics and antibiotic resistance genes in a sewage treatment plant and its effluent-receiving river. Chemosphere 119:1379–1385. doi: 10.1016/j.chemosphere.2014.02.040. [DOI] [PubMed] [Google Scholar]
- 56.Buchrieser C, Charpentier X. 2013. Induction of competence for natural transformation in Legionella pneumophila and exploitation for mutant construction. Methods Mol Biol 954:183–195. doi: 10.1007/978-1-62703-161-5_9. [DOI] [PubMed] [Google Scholar]
- 57.Costa J, Tiago I, Da Costa MS, Verissimo A. 2010. Molecular evolution of Legionella pneumophila dotA gene, the contribution of natural environmental strains. Environ Microbiol 12:2711–2729. [DOI] [PubMed] [Google Scholar]
- 58.Ruckdeschel G, Dalhoff A. 1999. The in-vitro activity of moxifloxacin against Legionella species and the effects of medium on susceptibility test results. J Antimicrob Chemother 43(Suppl B):25–29. doi: 10.1093/jac/43.suppl_2.25. [DOI] [PubMed] [Google Scholar]
- 59.Descours G, Ginevra C, Ader F, Forey F, Lina G, Etienne J, Jarraud S. 2011. Rifampicin-macrolide synergy against Legionella pneumophila serogroup 1 in human macrophages using a quantitative real-time PCR assay. Int J Antimicrob Agents 38:188–189. doi: 10.1016/j.ijantimicag.2011.05.001. [DOI] [PubMed] [Google Scholar]