Molecular analysis of fluoroquinolone-resistant salmonella paratyphi a isolate, India.
Salmonella enterica serovar Paratyphi A is the second most common cause of enteric fever after S. Typhi. Approximately 0.25 S. Paratyphi A infections (paratyphoid fever) occur for each S. Typhi infection (typhoid fever) (1). Given global estimates of >21 million cases of typhoid fever in the year 2000, >5 million cases per year of S. Paratyphi A probably occur. Paratyphoid fever is a major clinical problem in India, but large outbreaks were not reported until 1996 (2). Elsewhere, in southern China for example, extensive outbreaks are also occurring (3).
Since 1998, plasmid-mediated multidrug resistance in S. Paratyphi A, associated with chromosomally mediated reduced susceptibility to ciprofloxacin, has caused concern (4). Reduced susceptibility to fluoroquinolones results in a poor response of salmonellosis patients to treatment and may allow prolonged bacterial shedding (5). Rising resistance to fluoroquinolones is likely to be driving an increase in cases of paratyphoid fever in regions where fluoroquinolones are used empirically to treat enteric fever. We must monitor the emergence of resistance in this enteric pathogen to differentiate between the acquisition of resistance during treatment (mutations occurring in different bacterial strains) or clonal expansion of a successful strain by person-to-person spread (identical mutations associated with a single strain). To do so, we need to describe the molecular basis of resistance and the genotype of the resistant strains. High-level ciprofloxacin-resistant S. Paratyphi A (MIC 8 [micro]g/mL) is present in India (6) and Japan (MIC [greater than or equal to] 128 [micro]g/mL) (7). However, because S. Typhi, the major cause of enteric fever in India, has not yet developed high-level resistance to fluoroquinolones, enteric fevers are often treated empirically with fluoroquinolones. If this trend continues, fluoroquinolone-resistant strains of S. Paratyphi A are almost certain to become a major cause of enteric fever in many areas.
We analyzed, by DNA sequencing, the DNA gyrase and topoisomerase IV genes of the first reported highly fluoroquinolone-resistant S. Paratyphi A isolate (6). We looked at the full coding sequence, including the quinolone resistance-determining region (QRDR), of both subunits of DNA gyrase and topoisomerase IV for mutations associated with resistance to fluoroquinolones. We also used multilocus sequence typing (MLST) to confirm the identity of the isolate.
The strain described here (Pond1) was first isolated in Pondicherry, India, in November 2002 from the blood of a 23-year-old man admitted with fever and with no history of having received antimicrobial chemotherapy (6). The isolate was resistant to ciprofloxacin and nalidixic acid, and the MIC of ciprofloxacin was 8 mg/L. It was sensitive to all other antimicrobial drugs tested by disk diffusion: ampicillin, chloramphenicol, cotrimoxazole, gentamicin, and ceftriaxone. Repeat testing showed that zones of inhibition indicating susceptibility were seen around both ofloxacin (17 mm) and ciprofloxacin (21 mm) 5-[micro]g disks; however, in light of the ciprofloxacin MIC and resistance to nalidixic acid, Pondl was considered resistant to fluoroquinolones. No similar isolates have been seen in this area since the initial report, although the total number of paratyphoid fever cases has increased.
Polymerase chain reaction (PCR) amplification (Table 1) and direct DNA sequencing of both strands of the full length of gyrase (gyrA and gyrB) and topoisomerase IV (parC andparE) subunit genes was performed with an ABI Prism dye terminator cycle sequencing kit (Perkin Elmer, Foster City, CA, USA) on an ABI 3730 automated sequencer. Results showed 3 mutations: 2 in gyrA and 1 in parC. A comparison of these mutations with those previously described in fluoroquinolone-resistant S. Paratyphi A is shown in Table 2. A rise of fluoroquinolone resistance over time is apparent, and although the point mutations do not fully explain the MIC data, we noted general associations: a single mutation in gyrA is always associated with resistance to nalidixic acid and reduced susceptibility to ciprofloxacin and ofloxaein, and a double mutation in gyrA is always accompanied by mutations in parC and is associated with high-level (>4 [micro]g/mL) resistance. Although this sample is limited, heterogeneity in mutations found at all sites suggests that this finding is not the result of a single successful strain's sequentially acquiring mutations but rather that resistance is arising in several different strains.
The QRDR within topoisomerases contains hotspots for mutations around the active site, which are associated with raised MIC values for fluoroquinolones (10). For gyrA from nalidixic acid-resistant Salmonella isolates, 2 mutations are most frequently observed in clinical isolates: Ser83[right arrow]Phe and Ser83[right arrow]Tyr (8,9,11). The association with resistance of mutations seen in parC, however, is less clear (12). Mutations in parC of gram-negative bacteria are usually within the QRDR at amino acids 80 and 84 (Set 80[right arrow]Ile, Glu 84[right arrow]Gly, Lys). The first reported mutation was Thr57[right arrow]Ser, and other mutations have been described: Asp 79[right arrow]Ala, Gly 78[right arrow]Asp (9). Each mutation, in gyrA or parC, can give rise to different MICs in different isolates, which means that other factors must also influence the resistance phenotype in S. Paratyphi A. The most likely cause is changes in expression levels of proteins involved with permeability barriers and efflux pumps. These changes could be the result of either point mutations in transcription promoters and regulators or downstream effects of mutations in topoisomerases. Known mechanisms of fluoroquinolone resistance that we were able to screen for include transmissible plasmidborne resistance and efflux pumps. The qnr-containing plasmid was not detected with PCR using primers 5' GGG TAT GGA TAT TAT TGA TAA 3' and 5' CTA ATC CGG CAG CAC TAT TA 3' (13) in Pond1, and sensitivity testing gave the same zone size around both tetracycline and chloramphenicol discs when compared with a nalidixic acid-susceptible isolate. This finding, combined with the ciprofloxacin MIC of 8 [micro]g/mL, argues against the presence of multiple antimicrobial drug resistance efflux pumps. Thus the high-level resistance seen in Pond1 appears to be associated directly with 3 point mutations in the topoisomerase genes.
To confirm the identity of the isolate as S. Paratyphi A, we used MLST. The primer sequences and MLST data are available from the MLST database at the Max-Planck-Institut fur Infektionsbiologie (http://web.mpib-berlin. mpg.de/mlst/). Six of 7 sequenced loci matched exactly the previously described sequences, and 1 was a unique allele. This finding means that the isolate described here is within the clonal MLST group described as S. Paratyphi A but is a recognizable variant. This finding supports previous typing data that show very little variation (14); typing S. Paratyphi A is problematic because genomic restriction analyses (pulsed-field gel electrophoresis) of isolates from an outbreak are not always identical, and susceptible and resistant strains cannot be differentiated. For molecular epidemiologic studies to be carried out, several methods need to be used (15). A broader study of single base-pair differences between strains of S. Paratyphi A could provide a usable typing scheme.
Resistance in S. Paratyphi A populations must be monitored because the acquisition of resistance to fluoroquinolones, coupled with the reduction in S. Typhi by the use of typhoid-specific vaccination, may cause S. Paratyphi A to become the main cause of enteric fever. Disc susceptibility testing does not always detect resistance, and screening with nalidixic acid and MIC testing remains the method of choice. The isolate described here, Pond1, contains a unique combination of mutations that provides a way to track the spread of this strain of S. Paratyphi A.
We thank the diagnostic microbiologists who isolated and characterized the strains described in this manuscript.
Satheesh Nair, John Wain, and Keith Turner are funded by The Wellcome Trust of Great Britain.
Dr Nair is a research associate in tropical bacteriology at The Wellcome Trust Sanger Institute, The Wellcome Trust Genome Campus, United Kingdom. His research includes the use of molecular tools to detect genomic diversity of drug-resistant/drug-susceptible Salmonella spp. from different geographic and epidemiologic backgrounds and effects of drug resistance on the biology of the organism.
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Address for correspondence: Belgode Narasimha Harish, Department of Microbiology, JIPMER, Pondicherry 605006, India; fax: 91-413-2272067; email: email@example.com
Satheesh Nair, * Madhulika Unnikrishnan, (dagger]) Keith Turner, * Subash Chandra Parija, ([dagger]) Carol Churcher, * John Wain, * and Belgode Narasimha Harish ([dagger])
* The Wellcome Trust Sanger Institute, Cambridgeshire, United Kingdom; and ([dagger]) Jawaharlal Institute of Postgraduate Medical Education and Research, Pondicherry, India
Table 1. Primer sequences for amplification of topoisomerases Gene (coding sequence Primer Sequence 5'-3' Amplicon length) gyrA7 (F) 5' GGGTCGACTGATTATGGTTTATGCCTCC 3' 3199 2637 gyrA25 (R) 5' GAGACTTTCAGCGTAGTTCG 3' gyrB1 (F) 5' TTGCCTCTGAACTTGACGATGC 3' 2762 2415 gyrB9 (R) 5' GAAGTCGCTGACCTGCTCAC 3' parC3 (F) 5' CGATTTTCCGGTCTTCTTCCAG 3' 2616 2259 parC10 (R) 5' GCAATGCACGAATAAACAACGG 3' parE3 (F) 5' CCTGATCTGGCTACTGCAACAG 3' 2183 1893 parE8 (R) 5' ATGCGCAAGTGTCGCCATCAG 3' Table 2. Presence of gnr and mutations in DNA gyrase and topoisomerase IV genes of Salmonella enterica serovar Paratyphi A strains associated with decreased susceptibility or resistance to ciprofloxacin * MIC ([micro]g/mL) Country Year Cp Nal India 1999 0.38 >256 Bangladesh 1999 0.5 >256 India 1999 0.5 >256 Hong Kong 2000 0.5 >256 Japan 2002 [greater than or equal to] 128 >256 India 2002 8 >256 Country qnr gyrA India ND Ser83 [right arrow] Phe Bangladesh ND Asp87 [right arrow] Gly India ND Ser83 [right arrow] Phe Hong Kong ND Ser83 [right arrow] Tyr Japan ND Ser83 [right arrow] Phe, Asp8 [right arrow] Asn India NP Ser83 [right arrow] Phe, Asp87 [right arrow] Gly Country parC Reference India ND (8) Bangladesh ND (8) India ND (8) Hong Kong NM (9) Japan Glu84 [right arrow] Lys (7) India Ser80 [right arrow] Arg ([dagger]) This study * No mutations were detected in gyrB and parE. Cp, ciprofloxacin; Nal, nalidixic acid, ND, not determined; NP, not present; NM, no mutation within the quinolone resistance-determining region. ([dagger]) European Molecular Biology Laboratory accession no. AM050347.
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|Author:||Harish, Belgode Narasimha|
|Publication:||Emerging Infectious Diseases|
|Date:||Mar 1, 2006|
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