Department of Population Health and Pathobiology, College of Veterinary Medicine, North Carolina State University, 4700 Hillsborough St., Raleigh, NC 27606, USA
Received 19 May 2005; returned 28 July 2005; revised 3 August 2005; accepted 4 August 2005
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Abstract |
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Methods: Swine faecal and carcass swabs were collected from 10 groups of pigs (five each from intensive and extensive ABF farms) at the finishing farm and the slaughter plant. A total of 292 pigs at farm (extensive 118; intensive 174) and 254 carcass swabs (extensive 134; intensive 120) were collected during the study. Campylobacter species were isolated under microaerobic conditions and confirmed by biochemical testing. Up to three presumptive Campylobacter colonies per positive pig/carcass were further characterized. Speciation was done by PCR, targeting ceuE and hipO genes for Campylobacter coli and Campylobacter jejuni, respectively. The isolates were tested for their antimicrobial resistance profile using the agar dilution method against six antimicrobials.
Results: A total of 526 Campylobacter isolates were cultured from 292 pigs and 254 carcasses sampled. All the isolates were found to be C. coli. Overall prevalence of C. coli was 55.8% on farm (55% extensive and 56.3% intensive) and 26% at slaughter (32.8% extensive and 18.3% intensive). There was no significant difference in C. coli between the intensive and extensive systems on the finishing farms (P = 0.83). At post-chill stage, C. coli were isolated only from the extensively reared ABF pigs. Antimicrobial resistance against ciprofloxacin (MIC > 4 mg/L) was found at the farm level in both the intensive- and extensive-reared groups. The erythromycin/nalidixic acid/tetracycline resistance pattern (3%) was the most common pattern in multidrug-resistant C. coli.
Conclusions: This study highlights the high prevalence of diverse and antimicrobial-resistant C. coli in the ABF production systems of swine. This is the first study reporting the isolation of ciprofloxacin-resistant strains from ABF pigs in the USA and warrants concern.
Keywords: pig , Campylobacter species , antibiotic resistance , antimicrobial-free production
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Introduction |
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Studies on pigs reared in the conventional system of production where antimicrobials are used regularly for therapeutic and growth promotion have reported the prevalence of antimicrobial-resistant strains of C. coli.4,5 Studies of antimicrobial-free (ABF) production systems have been done before in the poultry industry in Europe.6 However, no study has been reported on swine reared in the ABF system in the United States. Under the ABF system of pig production, no antimicrobials were either added in the feed for growth promotion nor given for therapeutic purposes. Any pig that was treated for any infection was immediately removed from the herd. The primary objectives of the study were to determine the prevalence and antimicrobial susceptibility of Campylobacter isolates from the extensive (outdoor) and intensive (indoor) ABF production systems on-farm and at slaughter.
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Materials and methods |
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In the extensive ABF pig production system, pigs were reared in open fields in a barricaded area and had free access to the environment including soil and water. Under the intensive system, pigs were reared in confined barns with concrete slatted floors. A total of five finishing farms were sampled from each system over a period of 2 years from 2002 to 2004. At every farm visit, we sampled 30 pigs and collected 10 g of fresh faecal samples per rectum with gloved hands. Carcass samples were collected using sterile swabs soaked in 10 mL of buffered peptone water (Becton Dickinson, NJ, USA). Ten individual carcass samples were collected at each of the three processing stages: pre-evisceration, post-evisceration and post-chill. Carcass samples were collected by swabbing at the jowl, belly and the ham region. Pigs from the two ABF systems were slaughtered at two different slaughter plants. The intensively reared pigs were slaughtered in a slaughter plant with a blast chiller system for cooling the carcass in 2 h with a temperature of 30°C. The extensive pigs were slaughtered in a smaller plant using overnight chilling to cool the carcass (14°C for
18 h). The study protocol has been approved by the Institutional Animal Care and Use Committee.
Campylobacter isolation and speciation
Campylobacter isolation from the samples was done by directly plating a loopful of the sample onto campy-cefex selective plates and incubating under microaerobic conditions (CO2: 10%, O2: 5% and N2: 85%) at 42°C for 48 h. Up to three presumptive Campylobacter colonies per positive sample were selected for further analysis. Biochemical confirmation of colonies was done using the catalase (3% H2O2) and the oxidase tests (tetramethyl-p-phenylenediamine) (Becton Dickinson, NJ, USA).
PCR detection of C. coli and C. jejuni was done using species-specific primers. The ceuE and the hipO gene were used for detection of C. coli and C. jejuni.7 The forward and reverse primers for ceuE gene amplification were CC2, 5'-GATTTTATTATTTGTAGCAGCG-3' and CC3, 5'-TCCATGCCCTAAGACTTAACG-3' and for the hipO gene amplification were Hip1A, 5'-ATGATGGCTTCTTCGGATAG-3' and Hip2B, 5'-GCTCCTATGCTTACAACTGC-3', respectively. PCR thermocycling conditions were the same as described previously.7
Antimicrobial susceptibility testing
The agar dilution method was used to determine the susceptibility to six antimicrobials according to the NCCLS guidelines for MIC determination for Enterobacteriaceae.8 The antimicrobials (with their concentration ranges and breakpoints for resistance) were: chloramphenicol (0.25128 mg/L, 32 mg/L); ciprofloxacin (0.0084 mg/L, 4 mg/L); erythromycin (0.0632 mg/L, 8 mg/L); gentamicin (0.0632 mg/L, 16 mg/L); nalidixic acid (0.25128 mg/L, 32 mg/L); and tetracycline (0.0632 mg/L, 16 mg/L). C. jejuni ATCC 33560 was used as the quality control (QC) organism for this test.
Statistical analysis
Campylobacter prevalence and frequency were compared using the 2 test (Minitab Inc., PA, USA) and Fisher's exact two-tailed test wherever applicable. A value of P < 0.05 was considered statistically significant.
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Results |
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Campylobacter was isolated from all the farms and slaughter plants. The overall Campylobacter prevalence at the farm and slaughter level was 55.8% and 26%, respectively. Up to three isolates per positive sample (pig or carcass) were further analysed. All the 526 Campylobacter isolates in this study, including 366 from farm and 160 from slaughter, were C. coli. There was no significant difference in C. coli prevalence at the farm level for the extensive (55%) and intensive (56.3%) rearing systems (P = 0.83). However, a significantly higher proportion of C. coli was found at the pre-evisceration stage of processing extensively reared ABF pigs (P < 0.001). In both of the ABF systems, there was an increase in C. coli prevalence at post-evisceration followed by a significant decrease at the post-chill stage (P < 0.002). On comparing the two ABF systems at the post-chill stage, we observed C. coli only from the carcasses of extensively reared ABF pigs.
Antimicrobial resistance: frequency and patterns
We detected resistance to all of the six antimicrobials tested. Overall, isolates exhibited the highest frequency of resistance against tetracycline (48.6%) and erythromycin (39.7%) (Table 1). A significantly higher proportion of C. coli isolates from the intensive system were resistant to the above two antimicrobials at the finishing farms (P < 0.001). Resistance against ciprofloxacin (MIC > 4 mg/L; 0.5%) was detected in isolates from on-farm specimens and in both types of ABF herds (n = 3). Gentamicin- and chloramphenicol-resistant isolates were rare and observed in 0.2% and 1.9% of the total isolates, respectively.
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Discussion |
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Even though neither tetracycline nor macrolides were used as growth promoters in ABF herds, a significant proportion of isolates from the slaughterhouse, including post-chill samples, showed resistance against tetracycline and erythromycin. A high proportion of Campylobacter isolates showing resistance to these two antimicrobials has been reported before in pigs that were reared in the conventional production systems.3,5 None of the slaughterhouses where the samples were collected were dedicated for ABF herds. Thus, the likelihood of cross-contamination at lairage and processing remains a possibility. Resistance against ciprofloxacin was also detected at the farm level in the ABF production systems. Resistance against ciprofloxacin and chloramphenicol in C. coli is striking since both the antimicrobials are not licensed for use in any system of pig production in the USA. High resistance against ciprofloxacin has been reported in 100% of C. coli from pigs.3 The erythromycin/nalidixic acid/tetracycline resistance pattern was the most common MDR pattern in our study and has also been reported by Payot et al.5 to be the most common MDR pattern in their study. It should be noted that none of these antimicrobials (tetracycline and macrolides) or related classes of antimicrobials were used in any of the swine farms in this study.
In conclusion, this study highlights the prevalence of antimicrobial-resistant C. coli from both the extensive- and the intensive-type ABF production system. MDR ciprofloxacin-resistant C. coli isolates from swine is alarming since this antimicrobial is used in the treatment of severe invasive cases of campylobacteriosis. This study also indicates the possible role played by environmental factors in the dissemination of antimicrobial-resistant C. coli strains.
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Acknowledgements |
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References |
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