Bioscience Biotechnology Research Communications

An International  Peer Reviewed Refereed Open Access Journal

P-ISSN: 0974-6455 E-ISSN: 2321-4007

Bioscience Biotechnology Research Communications

An Open Access International Journal

Mohammad Hossein Sakhaie Shahreza1, Ebrahim Rahimi2* and Hassan Momtaz3

1Student of Veterinary Medicine, College of Veterinary Medicine, Shahrekord Branch, Islamic Azad University, Shahrekord, Iran

2Department of Food Hygiene and Public Health, College of Veterinary Medicine, Shahrekord Branch, Islamic Azad University, Shahrekord, Iran

3Department of Microbiology, College of Basic Sciences, Shahrekord Branch, Islamic Azad University, Shahrekord, Iran

Corresponding author Email: Ebrahimrahimi55@yahoo.com

Article Publishing History

Received: 15/05/2017

Accepted After Revision: 17/06/2017

ABSTRACT:

Shiga toxigenic Escherichia coli are the most important causes of food-borne diseases due to the consumption of contaminated ready to eat foods. The present investigation was done to study the prevalence rate and antibiotic resistance pattern of STEC strains recovered from various types of ready to eat foods. Seven-hundred and twenty various types of food samples were collected and cultured. Isolated E. coli strains were approved another time using PCR. Approved colonies were tested for antibiotic susceptibility using the disk diffusion. Twenty-six out of 720 food samples (5.20%) were positive for E. coli strains. Prevalence of STEC strains were 1.52%. Salad (15%) had the highest prevalence of bacteria, while hamburger (2.50%) had the lowest. STEC strains exhibited the highest levels of resistance against tetracycline (100%), ampicillin (100%), gentamicin (81.81%) and ciprofloxacin (72.72%), while exhibited the lowest against chloramphenicol (27.27%) and cotrimoxazole (45.45%). High prevalence of resistant STEC strains in ready to eat foods showed irregular prescription of antibiotic as well as lack of proper hygiene in restaurant and fast food centers. Cautious prescription of antibiotics and attentions to the principles of food security can decrease the risk of resistant STEC strains in ready to eat foods.

KEYWORDS:

Shiga Toxigenic Escherichia Coli, Prevalence, Antibiotic Resistance, Ready To Eat Foods

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Shahreza. M. H. S, Rahimi E, Momtaz H. Antibiotic Resistance Pattern of Shiga-Toxigenic Escherichia Coli Isolated from Ready-To-Eat Food Stuffs. Biosc.Biotech.Res.Comm. 2017;10(3).


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Shahreza. M. H. S, Rahimi E, Momtaz H. Antibiotic Resistance Pattern of Shiga-Toxigenic Escherichia Coli Isolated from Ready-To-Eat Food Stuffs. Biosc.Biotech.Res.Comm. 2017;10(2). Available from: https://bit.ly/2JpCHNS


Introduction

Food hygiene in restaurants and fast-foods are one of the most important critical issues in the society. Using from low quality raw materials, cooking of foods more than daily requirement and their storage in unsuitable conditions and finally lack in the observation of proper hygiene in cooking of foods are the main factors causing enhancement of microbial spoilage and growth of dangerous food-borne pathogens in foods (Isara and Isah, 2009). Among all pathogenic agents causing food-borne diseases and food poisoning, Escherichia coli (E. coli) strains had a significant importance (Momtaz et al. 2012; Momtaz et al. 2013). is a gram-negative, non-sporulating, flagellated, rod-shaped and facultative anaerobic bacterium which belongs to Enterobacteriaceae family. Shiga (vero) toxin (Stx)-producing E. coli (STEC) is a subdivision of an important pathogenic group of this bacterium named enterohemorrhagic E. coli (EHEC) (Momtaz et al. 2012; Momtaz et al. 2013; Dehkordi et al. 2014). STEC strains are responsible for intensive clinical syndromes like lethal hemolytic uremic syndrome (HUS), bloody and non-bloody diarrhea, thrombotic thrombocytopenic purpura (TTP) and hemorrhagic colitis (HC) (Momtaz et al. 2012; Momtaz et al. 2013; Dehkordi et al. 2014 and Ranjbar et al. 2017).

High levels of resistance in STEC strains is another important factor which increase the pathogenicity of bacteria. Unfortunately, STEC strains recovered from food stuffs and also cases of diarrhea and food poisoning harbored the high levels of resistance against commonly used groups of antibiotics including quinolones, aminoglycosides, macrolides, cephalosporins, sulfonamides, fluoroquinolones and tetracycline (Momtaz et al. 2013b; Momtaz et al. 2013c; Stewardson et al. 2014; Amézquita-López et al. 2016). In the other hands, STEC strains of food poisoning show a high incidence of resistance (85-100%) against commonly used antimicrobial agents (Momtaz et al. 2013b; Momtaz et al. 2013c; Stewardson et al. 2014; Amézquita-López et al. 2016).

Materials and Methods

The study was approved by the Ethical Committee of Islamic Azad University, Shahrekjord Branch (Consent Ref Number IAU 2053). Verification of this research project and the licenses related to sampling process were approved by the Prof. EbrahimRahimi (Approval Ref Number Food-Hygiene 95 2020). From September 2013 to September 2014, a total of 720 various types of ready-to-eat foods including sausage (n=70), salami (n=70), hamburger (n=60), roast mouthful (n=60), traditional dressing (n=65),traditional salad (n=60), traditional candy (n=60), traditional ice-cream (n=60), barbecue (n=70), soup (n=75) and spices (n=70) were randomly collected from various restaurant in the Isfahan province, Iran. Samples were immediately transferred to laboratory in cooler with ice-packs.

Totally, 10-g of crushed food samples were homogenized for 2 min in 90 ml of Peptone Water (PW, Merck, Germany). Then the samples were cultured on 5% sheep blood and MacConkey agar (Merck, Germany) and incubated for 18 to 24 h at 37 oC. Colonies with the typical color and appearance of E. coli were picked and streaked again on blood agar plates and re-streaked on EMB agar (Merck, Germany). All plates were further incubated for 24 h at 37 oC. The green metallic sheen colonies were considered as E. coli. The presumptive colonies were biochemically tested for growth on triple sugar iron agar (TSI) and lysine iron agar (LIA), oxidative/fermentative degradation of glucose, citrate utilization, urease production, indol fermentation, tryptophan degradation, glucose degradation (methyl red test) and motility. Bacterial strains were sub-cultured overnight in Luria-Bertani broth (Merck, Germany) and further incubated for 48 h at 37 oC. Genomic DNA was extracted from bacterial colonies using the DNA extraction kit (Fermentas, Germany) according to manufacturer’s instruction. Bacterial colonies were further confirmed using the 16S rRNA-based Polymerase Chain Reaction (PCR) (Woo et al. 2001) Set of primers used for this purpose are Forward: 5’-AGTTTGATCCTGGCTCAG-3’ and Reverse: 5’-AGGCCCGGGAACGTATTCAC-3’ (1343 bp). Prevalence of STEC strains was determined according to the method described by SafarpoorDehkordi et al. (2014) and Momtaz et al. (2013a).

Pattern of antimicrobial resistance was studied using the simple disk diffusion technique on Mueller–Hinton agar (Merck, Germany). Susceptibility of STECstrains were tested against tetracycline (30 u/disk), ampicillin (10 u/disk), cefotaxime (30 µg/disk), gentamycin (10 µg/disk), ciprofloxacin (5 µg/disk), cotrimoxazole(30 µg/disk), enrofloxacin(5 µg/disk), trimethoprim(5 µg/disk), and chloramphenicol (30 µg/disk) antibiotic agents (Oxoid, UK). All of the inoculated plates were aerobically incubated at 37 °C for 18-24 h. Results were interpreted based on the instruction provided by CLSI (2012) (Wayne 2012). E. coli ATCC 25922 was used as quality control.Statistical analysis was performed using SPSS/16.0 software for significant relationships. The incidence of antibiotics resistance of STEC isolated from various types of ready-to-eat food samples were statistically analyzed. Statistical significance was regarded at a value < 0.05. Results and Discussion

The present investigation was done in order to assess the prevalence of E. coli and STEC strains as well as study the antibiotic resistance pattern of isolated bacteria. Table 1 represents the total prevalence of E. coli and STEC strains isolated from various types of ready to eat foods. Twenty-six out of 720 food samples (5.20%) were positive for E. colistrains. Among all 26 E. coli strains, 11 strains (42.30%) were considered as STEC strains. Salad (15%), candy (12.50%) and barbecue (10%) were the most commonly contaminated samples. There were no positive results for Sausage, salami, roast mouthful and soup samples. Statistically significant differences were seen between the types of samples and prevalence of STEC strains (<0.05).

Table 1: Total prevalence of Escherichia coli and also STEC strains in various types of ready to eat food samples.
Types of samples No. samples collected No positive strains (%) PCR confirmation (%) STEC strains (%)
Sausage 70
Salami 70
Hamburger 60 1 (2.50) 1 (2.50) 1 (100)
Roast mouthful 60
Dressing 65 4 (8) 4 (8) 1 (25)
Salad 60 6 (15) 6 (15) 2 (33.33)
Candy 60 5 (12.50) 5 (12.50) 1 (20)
Ice cream 60 2 (5) 2 (5) 2 (100)
Barbecue 70 5 (10) 5 (10) 2 (40)
Soup 75
Spices 70 3 (5) 3 (5) 2 (66.66)
Total 720 26 (5.20) 26 (5.20) 11 (42.30)

Table 2 represents the antibiotic resistance pattern of STEC strains isolated from various types of ready to eat food samples. We found that STEC strains harbored the highest levels of resistance against tetracycline (100%), ampicillin (100%), gentamicin (81.81%) and ciprofloxacin (72.72%). Resistance against chloramphenicol (27.27%) and cotrimoxazole (45.45%) were low. Statistically significant differences were seen between the types of samples and prevalence of antibiotic resistance (p<0.05).

Table 2: Total distribution of antibiotic resistance pattern of STEC strainsisolated from various types of ready to eat food samples.
Samples (No. STEC strains) Antibiotic resistance pattern (%)
Tet* Amp Cef Gen Cip Cot Enr Tri C30
Hamburger (1) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100)
Dressing (1) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100)
Salad (2) 2 (100) 2 (100) 1 (50) 1 (50) 1 (50) 1 (50) 1 (50) 1 (50)
Candy (1) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100) 1 (100)
Ice cream (2) 2 (100) 2 (100) 1 (50) 2 (100) 1 (50) 1 (50) 1 (50) 1 (50)
Barbecue (2) 2 (100) 2 (100) 2 (100) 2 (100) 2 (100) 1 (50) 1 (50) 1 (50) 2 (100)
Spices (2) 2 (100) 2 (100) 1 (50) 1 (50) 1 (50) 1 (50) 1 (50) 1 (50)
Total (11) 11 (100) 11 (100) 7 (63.63) 9 (81.81) 8 (72.72) 5 (45.45) 6 (54.54) 6 (54.54) 3 (27.27)
*Tet: tetracycline (30 u/disk), Amp: ampicillin (10 u/disk), Cef: cefotaxime (30 µg/disk), Gen: gentamycin (10 µg/disk), Cip: ciprofloxacin (5 µg/disk), Cot: cotrimoxazole(30 µg/disk), Enr: enrofloxacin(5 µg/disk), Tri: trimethoprim(5 µg/disk), C30: chloramphenicol (30 µg/disk).

The present investigation showed that resistant STEC strains had a considerable prevalence in various types of ready to eat food samples. Total prevalence of E. coli and also STEC strains among the food samples of our study were 5.20% and 1.52%, respectively which emerged an important public health issue regarding the consumption of ready to eat foods.

There were some likelyexplanations for the high prevalence of E. coli and also STEC strains in the ready to eat food samples. At first. high-volume food production and long process of catering caused several problems such as lack of adequate precision and accuracy in the preparation and washing of raw materials and even their well cooking, lack of enough time and even temperature for cooking of raw materials, cooling of foods during processing, lack of reaching of sufficient heat to the center of meat and other food materials, lack of enough time to withdraw meat from the frozen state and finally cooking of meat and its products more than the daily requirement and then their storage at improper temperature and conditions. These mentioned circumstances maybe lead to survival and even growth of pathogenic microorganisms in ready to eat foods. At second, using from unsanitary and also contaminated equipment and dishes for production of foods in restaurant and fast food centers. At third, presence of infected staffs which maybe the sources of dangerous pathogenic agentsin the food processing stage (Shahrani et al. 2014; Hemmatinezhad et al. 2015; Ranjbar et al. 2017).

Sausage, salami and roast mouthful are mainly produced in high temperature and also they have been presented in a hygienic package. Therefore, it is not surprising that all of these samples were free from E. coli. High temperature using for cooking of soup make it clean from any pathogenic agents like E. coli. Because the large numbers of E. coliisolates recovered from raw meat, proper preparation of the raw meat can eliminate the distribution of bacteria. Unfortunately, principles of meat inspections were not observed in Iranian slaughterhouses. Therefore, close contact of animal carcasses with each other and even slaughterhouse floor, blood, content of the digestive tract and wool and skin of slaughtered animal caused transmission and distribution of pathogenic agents like E. coli to meat of slaughtered animals. Besides, the role of possible colonizers such as meat inspectors, butchers and miscellaneous people which mainly have come into the slaughterhouse for buying of meat and finally animals like rats, cats and birds which have been entered from outside the slaughterhouse as a sources of pathogenic E. coli should not be overlooked. Survival of STEC strains of raw food samples even after cooking procedure and occurrence of cross contamination after cooking procedure are two important routes of hospital foods contamination (Shahrani et al. 2014; Hemmatinezhad et al. 2015; Ranjbar et al. 2017).

High prevalence of resistance against commonly used antibiotic agents is another important finding of this study. We found that STEC strains harbored the high levels of resistance against tetracycline, ampicillin, cefotaxime, gentamycin, ciprofloxacin, cotrimoxazole, enrofloxacin, trimethoprim and chloramphenicol antibiotics. Indiscriminate and unauthorized prescription of antibiotics especially in the field of veterinary caused such high prevalence of antibiotic resistance in STEC strains recovered from foods (Shahrani et al. 2014; Hemmatinezhad et al. 2015; Ranjbar et al. 2017).

Several studies have been done in this field in various parts of the world. Miri et al. (2014) reported that from a total of 190 food samples, four samples (2.1%) were contaminated with E. coli. All of the E. coli strains were isolated from hamburger samples (3.3%). They found that all isolates (100%) were resistant to one or more antimicrobial agents and especially tetracycline and ampicillin.Srinivasan et al. (2007) showed that all of the E. coli strains of food samples exhibited resistance to five or more antimicrobial agents and especially ampicillin, aztreonam, cefaclor, cephalothin, cinoxacin, and nalidixic acid which was similar to us. Kalantar et al. (2013) reported that a total of 87 E. coli strains were detected from 466 rectal swabs from children with acute diarrhea and 40 E. coli strains were detected from the 125 frozen food samples of animal origin. They showed that consumption of contaminated foods may play an important role in occurrence of E. coli infections in children. Stewardson et al. (2014) reported that the prevalence of susceptibility of E. coli strains of food samples against meropenem, gentamicin, ciprofloxacin, cotrimoxazole, and fosfomycinin Switzerland were 100%, 90%, 87%, 79%, and 98%, respectively.

Conclusion

In conclusions, we identified a large number of STEC strains which were resistant against several types of antibiotic agents. Resistance against ampicillin, gentamycin andtetracycline and presence of multi-drug resistant strains were the most commonly detected characters in the STEC strains of ready to eat foods. It seems that there were no severemanagements on the principles of food hygiene in Iranian restaurant and fast food centers. Due to the low levels of STEC resistance against chloramphenicol and cotrimoxazole, occurrence of food poisonings due to the STEC strains in tested Iranian restaurant and fast food centers can be treated with their regular prescription. Attentions to the results of disk diffusion method and principles of hazard analysis and critical control point (HACCP) system can reduce the risk of STEC strains in food stuffs.

Acknowledgements

The authors would like to thank Prof. Amir Shakerian at the Department of Food Hygiene, Shahrekord Branch, Isamic Azad University, Shahrekord, Iran for his important technical support. This work was supported by the Islamic Azad University, Shahrekjord Branch (Ref Number IAU-Bud-177)

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