Occurrence and Antibiogram of Escherichia coli O157 : H7 in Raw Beef and Hygienic Practices in Abattoir and Retailer Shops in Ambo Town, Ethiopia

Foodborne infections are widespread and growing public health problems in the world. Shiga toxin-producing Escherichia coli O157 : H7 is one of the most significant foodborne pathogens. This study was conducted to assess the occurrence and antibiogram of E. coli O157 : H7 from raw beef as well as hygienic and sanitary practices of meat handling in abattoir and retailer shops. Systematic random sampling technique and census methods were used to collect samples from abattoir and retailer shops, respectively. All tryptone soya broth preenriched carcass samples were subcultured onto MacConkey agar. Then, the bacterium confirmed as Escherichia coli using biochemical tests was streaked onto Sorbitol-MacConkey agar and incubated at 37°C for 24 hrs. Escherichia coli O157 : H7 was confirmed by latex agglutination kit. In vitro antimicrobial susceptibility test of Escherichia coli O157 : H7 isolates was done against 13 antimicrobials. Hygiene and sanitation data were collected using a pretested structured questionnaire and observational checklist. Pearson Chi-square and Fisher's exact two-tailed tests were performed and differences were considered significant at P ≤ 0.05. Out of 197 meat samples, 23.4% (95% confidence interval (CI): 17.6–29.9%) and 9.1% (95% CI: 5.5–14.1%) were contaminated with Escherichia coli and Escherichia coli O157 : H7, respectively. There was a significant variation in the occurrence of Escherichia coli O157 : H7 between retailer shops (19.1%) and abattoir (7.2%) (P = 0.03). The study revealed that the municipal abattoir and retailer shops in Ambo town did not adhere to the required sanitation and hygienic standards. All Escherichia coli O157 : H7 isolates were susceptible to norfloxacin, sulfamethoxazole-trimethoprim, chloramphenicol, and ceftazidime. However, all isolates were resistant to amoxicillin. Multidrug resistance was widespread and was found in 66.3% of Escherichia coli O157 : H7 isolates. The occurrence of Escherichia coli O157 : H7 was high. Therefore, fulfilling national and international meat safety requirements, training and monitoring of meat handlers, and rational use of antimicrobials are recommended


Background
Foodborne diseases remain a challenging problem causing great human suffering and significant economic losses. While the burden of foodborne diseases is a public health concern globally, developing countries have the highest incidence and highest death rates [1]. e actual number of Escherichia coli (E. coli) O157 : H7 infections attributable to meat is difficult to assess accurately, because of the lack of diagnostic facilities and only a small proportion of illness cases are officially reported especially in developing countries [2]. However, a review of 16 articles and databases from 21 countries in Africa reported that the estimated global burden of E. coli O157 : H7 is 2,801,000 acute illnesses, 3890 cases of hemolytic uremic syndrome, and 230 deaths annually [3]. Foodborne diseases often follow the consumption of contaminated foodstuffs, especially from animal products such as meat from infected animals or carcasses contaminated with pathogenic bacteria [4]. Escherichia coli is among the most challenging Enterobacteriaceae group of bacterial meat contaminant worldwide. Most E. coli strains do not cause diseases and are actually part of the normal flora of the intestinal tract of animals and humans but detection of E. coli in foods intended for human consumption shows poor sanitary and hygiene during production, processing, transportation, or preparation [5]. However, there are a number of different pathogenic groups of E. coli that have been shown to cause various types of gastrointestinal infections, and deaths have been observed in humans. Among the enteric E. coli, shiga toxin-producing E. coli O157 : H7 is the most significant foodborne pathogens that have gained increased attention in recent years [6]. It has been the most commonly isolated serotype in association with abdominal cramps, bloody diarrhea, thrombotic thrombocytopenic purpura, hemorrhagic colitis, and hemolytic uremic syndrome in both outbreaks and sporadic cases [7].
Ruminants are regarded as the main reservoir of E. coli O157 : H7 though it has been isolated from other animal species such as pigs, gulls, geese, and pet animals [8]. Food is the predominant transmission route of E. coli O157 : H7 which is responsible for more than 52% of outbreak-related cases in the United States. Beef is the most common vehicle among foodborne outbreaks of E. coli O157 : H7 [9]. It can be contaminated through contact with the animal's skin and hair, limbs, blood, stomach, gut contents, bile and, equipment, hands, and worker's clothes [10]. Bacterial contamination of the feces/hide can be transferred onto previously sterile meat surfaces during slaughtering and dressing especially when slaughtering is performed on the floor with the absence of a carcass suspension system and careless evisceration that spreads intestinal content onto the meat surface [11].
Resistance to antimicrobial is highly prevalent in bacterial isolates worldwide, particularly in developing countries [12]. Antimicrobials are used in food animals to prevent, control, and treat disease and to promote the growth of food-producing animals. e increased use of antimicrobial agents in food animal production and human is a significant factor in the emergence of antimicrobialresistant bacteria [13]. A review of 40 years of enteric antimicrobial resistance research in Eastern Africa states that E. coli O157 : H7 is potential for zoonotic transmission to humans and has developed high rates of resistance to available treatment regimens [14]. Meat is a major source of transmission of antimicrobial-resistant organisms to humans causing disease [15]. Furthermore, this situation is complicated by the potential of resistant bacteria to transfer their resistance determinants to resident constituents of the human microflora and other pathogenic bacteria [15,16].
In developing countries, there is a food safety knowledge gap and animals are commonly slaughtered and dressed under unhygienic conditions [17,18]. Ethiopia is one of the developing sub-Saharan African countries sharing the high burden of diarrheal morbidity and mortality [19]. Information about human infections with E. coli O157 : H7 is limited in this country; nevertheless, in a study conducted on 422 diarrheic children under 5 years in the northern part of Ethiopia, 59 (28.9%) of the children were positive for E. coli O157 : H7 [20]. e habit of consuming raw and/or undercooked meat is one of the factors that exacerbate the transmission of foodborne pathogens including E. coli O157 : H7 in the country. Sufficient heating of meat kills these organisms [21]. However, consumption of raw or undercooked beef in the form of "kitfo" (minced raw beef mixed with a chili powder-based spice blend and a clarified butter infused with herbs and spices), "leb-leb" (undercooked "kitfo"), "gored-gored" (cuts of raw meat with butter and pepper), and "kurt" (raw beef consumed with hot pepper and mustard) is common cultural practices in Ethiopia [22].
In Ethiopia, the few studies conducted on E. coli O157 : H7 showed prevalence ranging from 2.3% to 10.4% [22][23][24][25]. However, studies on the hygiene and sanitation practices in meat processing establishments are lacking. erefore, the aim of the present study was to investigate the prevalence of E. coli, occurrence and antibiogram of E. coli O157 : H7 from raw beef, and hygienic and sanitary practices of meat handling in abattoir and retailer shops in Ambo town, West Shewa Zone, Ethiopia.

Study Design and Study Area.
A cross-sectional study design was employed for the purpose of this study. ere are 31 legally registered retailer shops and 1 municipal abattoir in Ambo town during the study period. All retailer shops receive carcass from Ambo municipal abattoir. Ambo town is the administrative center of West Shewa Zone. It is located at latitude and longitude of 8°59′N 37°51′E8.983°N 37.85°E, respectively, and at an elevation of 2101 meters above sea level and 114 Km West of Addis Ababa, the capital of Ethiopia.

Sample Size Determination.
Sample size for this study was determined using single population proportion standard formula.
Z is z statistic for level of confidence, n is the required sample size, P is the expected prevalence, and d is desired absolute precision. Previous study done in abattoir and retailer shops in Addis Ababa showed the prevalence of E. coli O157 : H7 to be 13.3% [22]. erefore, using 13.3% expected prevalence, at a confidence level of 95% and required absolute precision of 5%, the minimum calculated sample size was 174. But 197 samples were taken deliberately in order to maximize the precision of the study. Out of the total samples collected, 166 and 31 meat samples were from Ambo municipal abattoir and retailer shops, respectively.

Questionnaire Survey.
A pretested structured questionnaire and observational checklists were used to collect the necessary field-level data. ey were designed after reviewing 2 Veterinary Medicine International relevant literature, national and international guidelines to obtain hygienic status, and practices in abattoir and retailer shops. Structured questionnaire interview was used to collect data from 31 retailers (one from each retailer shop) and all 14 abattoir workers who are directly involved in slaughtering, evisceration, and carcass splitting. e questionnaire was developed to gather data about sociodemographic characteristics, meat handling experience, training on meat safety, status of medical screening and certification, knowledge about foodborne disease, and hygienic practices of workers regarding meat safety in the abattoir and retailer shops. Observational checklist was used to collect data regarding housing (floor, roof, and ceiling) of retailer shops and abattoir, availability of cooling materials, tap water, hot water, retention room, and bathroom in meat handling places. Additionally, practices like slaughtering, evisceration, splitting, loading, and transportation of carcass in the abattoir were included.

Sample Collection
Procedure. First, animals were selected using a systematic random sampling technique from a list of animals that were brought to Ambo municipal abattoir. en, raw cut of meat samples was collected from specific sites (neck, brisket, fore rib, flank, and rump) of a carcass [26]. Similarly, raw meat samples from the same sites of carcasses were collected from all meat retailer shops in Ambo town (n � 31). All samples from different retailer shops and abattoir were placed in separate sterile plastic bags (Seward, England), labeled with identification number, and immediately transported to the Ambo University Zoonoses and Food Safety Laboratory in an icebox with ice packs and processed within 4 hrs.

Sample Preparation and Isolation
Procedure. Raw meat samples collected from abattoir and retailer shops were taken out of plastic bags using sterile thumb forceps. From each chopped and mixed meat sample, 25 gm was transferred into a sterile stomacher bag (Seward, England), containing 225 ml of tryptone soya broth (TSB) (Himedia, India) and homogenized using homogenizer (Stomacher 400, Seward Medical, England) at 260 RPM for 2 minutes. e resulting homogenate was incubated at 37°C for 24 hrs. All preenriched meat samples were subsequently subcultured onto MacConkey agar (Himedia, India) and incubated at 37°C for 24 hrs. Five to ten suspected colonies of E. coli (pinkish color appearance) were subcultured onto separate nutrient agar (Himedia, India) and confirmed by biochemical tests: fermentation of lactose and glucose using triple sugar iron agar, hydrogen sulfide (H 2 S) negative, production of indole (positive), methyl red test (positive), Voges-Proskauer test (negative), and Simon citrate agar test (negative) were considered as E. coli.
en the bacterium confirmed as E. coli was streaked onto Sorbitol-MacConkey agar (Himedia, India) and incubated at 37°C for 24 hrs. Nonsorbitol fermenting (colorless) isolates were passed for serological typing.
2.6. Serological Test. All nonsorbitol fermenting colonies from the Sorbitol-MacConkey agar were serologically confirmed using E. coli O157 : H7 latex agglutinations assay (Abraxis LLC, USA), containing latex particles coated with antibodies specific for E. coli O157 : H7 antigen. Identification of E. coli O157 : H7 was carried out following the manufacturer's instruction. Nonsorbitol fermenting isolates were inoculated onto nutrient agar for serological testing. Using one of the provided transfer pipettes, one drop of peptone buffered saline (PBS) was placed onto one (1) circle on the test card. A portion of a suspected colony from the agar plate was picked using single used sterile plastic sticks and emulsified thoroughly in the drop of PBS in one of the circles. One free falling drop (with vial held vertically) of the E. coli O157 : H7 Latex Antibody bead reagent was dispensed onto each circle and the test card rotated using a complete circular motion for up to one minute or until agglutination was evident; whichever occurs first, the results were recorded. Agglutination of the test latex within one minute was considered as a positive result.
is indicates the presence of E. coli serogroup O157 : H7. e absence of agglutination occurring within one minute was considered a negative result.
is indicates the absence of E. coli serogroup O157 : H7.

Antimicrobial Susceptibility
Test. E. coli O157 : H7 isolates were subjected to in vitro susceptibility test against 13 commonly used antimicrobial drugs using the disk diffusion method following guidelines established by the Clinical and Laboratory Standards Institute (CLSI) [27]. Test suspension was prepared from a pure culture of E. coli O157 : H7 isolates, inoculated into a test tube of 5 ml TSB (Himedia, India), and incubated at 37°C for 6 hrs. e bacterial suspension was adjusted to 0.5McFarland turbidity standards. Mueller-Hinton agar (Bacton Dickinson, USA) plates were prepared according to the guidelines of the manufacturer. e diluted bacterial suspensions were swabbed in three directions uniformly on the surface of Mueller-Hinton agar plates using sterile cotton swabs. After the plates dried, with the aid of sterile thumb forceps, antibiotic-impregnated disks (Oxoid, England) were placed to the surface of the inoculated plates. en, the plates were incubated aerobically at 37°C for 24 hrs. Finally, the diameter of the inhibition zone formed around each disk was measured on black surface using a transparent ruler by placing it over the plates. e results were classified as sensitive, intermediate, and resistant according to the CLSI [27].

Quality Control.
Confidences in the reliability of test results were increased by adequate quality assurance procedures and the routine use of control strains. us, E. coli ATCC-25922 (susceptible to all tested drugs) was taken as an important part of quality control for culture and antimicrobial susceptibility tests. e sterility of sample collecting materials was checked randomly by culturing on nutrient agar and sterility of culture media was checked by incubating from each batch of prepared media for 24 hrs. Moreover, the whole procedures and result interpretation were done following standard operating procedure (SOP). e questionnaire was daily checked by the principal investigator for its completeness.
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Data Management and Statistical Analysis.
Questionnaire and laboratory data were entered into a Microsoft Excel spreadsheet. SPSS 20 statistical software (SPSS Inc., Chicago, IL, USA) was used for analyses of data. Descriptive statistics such as frequencies were used to present the findings of the questionnaires. e percent occurrence of E. coli O157 : H7 in beef samples was estimated using a formula, that is, the number of positive samples divided by the total number of samples examined multiplied by 100. e binomial exact method was used to calculate the 95% confidence interval (CI) of the prevalence estimates. P-value ≤ 0.05 was considered statistically significant.

Sociodemographic Characteristics of Retailer Shops and Abattoir and Workers.
e results of the sociodemographic information of abattoir and meat retailer men interviewed in the abattoir and retailer shops in Ambo are shown in Table 2.
e results revealed that all personnel working in the establishments are male. Most of the respondents from abattoir (42.9%) and from retailer shops (41.9%) were between the ages of 21 and 30 years.

Professional Experience, Training, Health Evaluation, and Awareness about Foodborne Disease of Study Participants.
Information regarding medical test, training, and professional experience of the interviewed workers is shown in Table 3. e majority (64.5%) of respondents did not know about their health status whether they are healthy enough to work in meat processing. More than half of the abattoir workers (54.8%) and meat retailer men (57.1%) have been working in the establishments for less than six years. e majority of retailer shops (83.5%) and abattoir workers (71.4%) did not receive formal training for sanitary and hygienic handling of meat.

Personal Hygiene and Sanitation of Workers regarding
Meat Safety. All the respondents from retailer shops indicated that they always clean their hands before meat handling and use reusable cloth towel to clean equipment and dry hands. About 35.5% of the respondents indicated that they do not wear a gown, but instead wear casual (street) clothes. About 51.6% of the respondents indicated that they do not remove their jewelry during meat handling. Most of the study participants (83.9%) wash their hands using cold water and soap. Similarly, 83.9% of respondents wash equipment (knife, ax, balance, etc.) every day at the end of the process. Seventy-four percent of the meat retailers wash meat using cold water when there is visible contamination, whereas 25.8% of them do not wash even if there is contamination, either they cut and remove or leave it as it is (Table 4).

Facilities and Hygienic Practices in Ambo Municipal
Abattoir.
e surroundings of abattoir house were full of leftover dirty materials and doors were always open without any restriction on personal movement to go inside and out of slaughterhouses. e floor of abattoir was made of concrete and impervious but has no ceiling. ere was no hot water, adequate supply of tap water, sterilizer, retention room (cooling facilities), change rooms, and bathroom facilities in the abattoir. Evisceration and carcass splitting takes place on the floor often not clean (Figure 1). Animals were not washed before slaughtering and there was no separation between dirty and clean areas in the abattoir. Workers were not interested in washing their hands, knife, and axes during slaughtering process and they were not interested in preventing leakage from the anus or bursting of the visceral contents to sterile carcass. ere is one meat inspector, but slaughtering happens in the absence of the meat inspector.
From total of 18 E. coli O157 : H7 isolates, 12 (66.3%) were found to be resistant to three or more antimicrobial drugs, that is, multiple drug resistance (MDR). e most frequently observed resistance combinations were cefuroxime and amoxicillin (33.3%) ( Table 5).

Discussion
e present study was conducted to assess the occurrence of E. coli O157 : H7 and its antimicrobial susceptibility on meat samples collected from an abattoir and retailer shops in Ambo town. e carcass contamination with E. coli in the retailer shops and abattoir was 23.4%. is is in agreement with the result of 24.8% reported in Dire Dawa [28] and 27.3% in Mekele municipality abattoir in northern Ethiopia [17]. e prevalence of E. coli in the present study was lower than the 46.5% reported in Nigeria [29].
Even though the present finding is lower than the report from Nigeria, it confirmed the high rate of contamination of meat with E. coli due to unhygienic practices, which is also an indication of the presence of unacceptable levels of other pathogenic microorganisms. 4 Veterinary Medicine International e occurrence of E. coli O157 : H7 (9.1%) from bovine meat at both the abattoir and raw meat retailer shops was in line with the previous study from Tigray 10.4% [30], Debre Zeyit 8% [23], and Addis Ababa 10.2% [22]. Additionally, comparable results were also reported in other parts of the world such as 8.9% [31] and 9.6% [32] in Iran, 8.8% [33] in South Africa, and 13.3% [34] in China.
However, the present finding is higher than some other reports from Ethiopia, such as 1.3% in Addis Ababa [25], 2.7% in Haramaya University [24], and 6.7% in Mekele [35],   Veterinary Medicine International and also from other countries in the world, such as 3.76% in Botswana [36], 1% in Ireland, 0.3% in the Czech Republic, and 0.3% in the Netherlands [37]. On the other hand, other scholars reported much higher results than the present findings: 60% from street meat sellers in Mekele town and 19.8% and 53% in Nigeria [38]. e overall variations in the prevalence of E. coli O157 : H7 might be due to the difference in sample size, sampling techniques, laboratory methodologies, study areas, time, and hygienic conditions employed [26,39]. With regard to meat, the source of the significantly higher contamination of E. coli O157 : H7 was found at the retailer     Veterinary Medicine International they clean the vehicle daily, it was not clean as per our observation. Abattoir workers carry the meat on their back or hold it using their two hands supporting through their chest. erefore, a higher prevalence of E. coli O157 : H7 at the retailer shops could be as a result of unhygienic handling practice of meat at retailer shops and direct contact between contaminated clothes of workers and carcass. Furthermore, there is a great possibility of bacterial cross-contamination due to direct contact of different carcasses while transporting together in a single vehicle.
e current study noted that 64.5% of workers in both abattoir and retail shops had no medical test and health certificate. Similar reports from Mekele [17] and Egypt [40] also noted that upon inspection most workers did not have valid health certificates. Shortcomings observed in the implementation of personal hygiene practices can be addressed by proper training, education, and monitoring of the workers [41]. In addition to this, regular updating and refresher courses should be carried out more frequently. is will help the meat handlers to have a better understanding of risks associated with contamination of meat with potential pathogens and sanitation practices [42]. Most respondents (83.9%) in the present study did not receive any formal training regarding hygiene and sanitation of meat handling neither prior nor after employment. is critical violation is comparable to the proportions of respondents of other studies who also indicated that they did not receive training [41,43]. Reports from Pretoria, South Africa [43], Western Romania [41], and Alexandria, Egypt [40], have shown that most meat handlers lack meat safety knowledge and adequate training and are frequently engaged in poor handling practices. Studies also highlighted that individuals with proper professional training regarding meat safety significantly do better practices compared to the untrained [41,42].
is shows that the quality of practices is improved mainly by professional training.
Meat contamination during processing is partly due to a lack of knowledge as to how to improve conditions in meat industry [44]. About 45.5% of the retailers and 64% of the abattoir workers knew that contaminated meat can cause bacterial diseases.
is study showed that 32.3% of retail workers and 57.1% of abattoir workers were able to name foodborne bacterial diseases and some of their signs and symptoms. Workers are at risk of meat contamination and should self-report when ill [44]. In this study, a large proportion of meat handlers from retailers (38.7%) and abattoir (42.9%) did not report any illness to the supervisors. Another previous study showed that 96.4% of the respondents report their illness to supervisors and visit the nearby health facility timely to get appropriate diagnosis and treatment [43], whereas in the present study 61.3% of the retailer and 57.1% of abattoir workers indicated that they go to clinic or hospital when sick. Reporting and taking a leave when sick is very important when working on the food premises to prevent chances of contamination [44]. However, in our study, as most of the participants were temporary workers paid on a daily basis, they were unlikely to report illness and take time off. ese conditions can lead to pathogen contamination of meat from meat handlers.
Contamination of meat and meat handlers could be prevented by wearing protective clothes [45]. About 35.5% of the respondents indicated that they did not wear protective clothing. Out of those who wear protective clothes, 30% of respondents' clothes were not clean. Haileselassie et al. [17] also recorded that a larger proportion of workers from selected butcher shops in Ethiopia operate without wearing protective clothing. In Kenya, less than 50% of workers wore protective clothing at all times [46]. In contrast to our study, Nel et al. [43] reported that all respondents declared that they always wear protective clothes. Working clothes should be cleaned every day [47]. However, in this study, only 27.5%, of respondents indicated that they wash their protective clothing daily. erefore, the workers need to be properly trained and provided with adequate protective clothing in order to prevent possible chances of crosscontamination.
In this study, all respondents indicated that they always clean their hands before meat handling. In addition, upon asking the workers what they use for handwashing, 83.9% indicated that they used soap and cold water. Damp hands can result in skin excoriation leading to a higher number of types of bacterial colonization and facilitate the spread of pathogens [48]. Our observation during the study showed that the retailer operators retailing meat also wiped their hands, cutting board, and scale surfaces with a dirty reusable cloth. e piece of cloth used was not frequently washed or changed during the day. Even though the intention was good, the wiping cloth was reused the whole day and can accumulate microorganisms that can be transferred to the retailer operators' hands, to utensil surfaces, and finally to meat. Soft, absorbent paper towels are recommended for drying hands than the use of a cloth. Clothes have been reported to be ineffective in removing microorganisms, thereby increasing the chance of cross-contamination [49].
In the current study, the majority (93.5%) of retailer shops' floor was constructed of concrete. All of the walls of the shops were painted with white and red color. Nevertheless, 35.5% of the retailer shops floor had cracks, and 19.4% of the shops do not have a ceiling which further hinders cleaning.
ese conditions in the present study settings disagree with the WHO and FAO standards [50]. e surrounding of the slaughterhouse is full of leftover dirty materials (gastrointestinal content, horn, shank, and bones) collected from daily slaughtered animals. Moreover, gates of abattoir are always opened without any restriction on personal movement to go inside and out of slaughterhouses.
is may create a favorable condition for transferring E. coli O157 : H7 from the environment to slaughterhouse.
e floor of the abattoir should be hard concrete and impervious, to reduce dirt in the slaughterhouse and allow drainage and ease of cleaning. Similarly, a roof is important to protect the carcass from the weather and to reduce the temperature in the slaughterhouse [50]. In the present study, floor of the abattoir is made of concrete and impervious but has no ceiling. Even though washing of the abattoir floor takes place every day at the end of slaughtering process, the wall is not cleaned and washed at the end of the working day. 8 Veterinary Medicine International According to international guidelines, hot and cold water, sanitizer, and retention room should be readily accessible for cleaning equipment and workers' hands [51].
ere were no hot water, adequate supply of tap water, sterilizer, retention room (cooling facilities) change rooms, and bathroom facilities in Ambo abattoir. From the observations made in the current study, there is no separation between dirty and clean areas. Both slaughter and postmortem operation are conducted in the same place and bleeding evisceration and carcass splitting take place on the ground in the same area, which leads to high possibilities of contamination during dressing of carcass from the skin, the intestines, and the ground. is is contrary to the recommendations of the Codex Alimentarius Commission [51] and Norrung and Buncic [52]. Any visual contaminations on the carcasses were removed by washing.
Unlike the reports of Gill et al. [53], Nastasijevic et al. [54], and Blagojevic et al. [55], this study confirmed that there was no washing of animals before slaughtering, "bagging" of anus and tying "rodding" of esophagus before evisceration. Feces adhering to the animals can be carried into the abattoir on the hair, hide, hooves, and tail of the animal and can become a major source of carcass contamination. Additionally, workers in the abattoir had no intention for personal hygiene and were not interested in washing their hands, knife, and axes during the slaughtering process. ey were not concerned to prevent leakage from the anus or bursting of the visceral contents to sterile carcass. eir hands and clothes were not clean throughout the working days.
Even though there is one veterinary meat inspector in the abattoir, it was observed that many of the activities in the abattoir happen in the absence of the meat inspector. is is in violation of the stipulations; a licensed inspector must perform antemortem and postmortem inspection and must be present when slaughtering is being conducted for meat intended for commercial purposes [56].
Antimicrobial resistance has been recognized as an emerging worldwide problem in human and veterinary medicine in both developed and developing countries. e increased use of antimicrobial agents in food animal production and human is a significant factor in the emergence of antibiotic-resistant bacteria [13]. Antimicrobial resistance of E. coli O157 : H7 isolates from animal and human sources have been reported from central Ethiopia [23]. In the present study, all of the 18 isolates were susceptible to norfloxacin, trimethoprim-sulfamethoxazole, chloramphenicol, and ceftazidime. is is consistent with the findings of Rahimi and Nayebpour in Iran [57] and Bekele et al. [22] in Ethiopia. On the other side, the current study revealed that isolates were resistant to amoxicillin (100%), cefuroxime (94.4%), ciprofloxacin (66.7%), amoxicillin-clavulanate (55.5%), tetracycline (27.7%), and gentamicin (22.2%). A study carried out in Saudi Arabia revealed a similar finding that there was a resistant strain to the drugs such as tetracycline and ciprofloxacin. A similar percentage of resistance to amoxicillin and tetracycline has been reported previously in Ethiopia [24]. e significantly high level of antimicrobial resistance was probably an indication of their extensive usage either in the public health sector or in the foodproducing animals or both for the therapeutic purpose of E. coli and other infections.
Multiple antimicrobial resistance may be acquired through mobile genetic elements such as plasmids, transposons, and class 1 integrons [58]. e present study showed that 66.3% of the E. coli O157 : H7 isolates were resistant to three or more classes of antimicrobials.
is finding was lower than the previous findings in Addis Ababa [25] and in Mekele [30]. Additionally, it was lower than with the findings of other researchers, who reported MDR among E. coli O157 : H7 isolates [59][60][61]. e occurrence of MDR in this study was higher than the findings of other studies conducted in Addis Ababa (22.6%) [23].
is finding is comparable to the previous finding in Haramaya (66.7%) [24]. e occurrence of MDR observed in this study might be due to the administration of multiple antimicrobials for prophylaxis or infection control and indiscriminate use of antimicrobials in the farms and/or public health sector, thereby selecting for resistant populations of E. coli O157 : H7.
e occurrence and multidrug resistance of E. coli O157 : H7 in this study imply an unacceptable level of hygiene and sanitation practice in meat handling and irrational use of antimicrobials. e high contamination of meat by MDR E. coli O157 : H7 and widespread habit of raw beef consumption in Ethiopia [22] call a concern for a potential outbreak of drug-resistant human pathogens for customers who regularly consume raw meat in the study area.

Limitation of the Study
Quantitative analysis of microbial load of meat in the abattoir and retailer shops was not performed. Isolation of E. coli O157 : H7 was done without selective enrichment and selective media. e result in this study indicates a relatively high frequency of E. coli 157:H7. However, the percentage of E. coli 157:H7 reported in this study might be an underestimate due to the chances of losing the specific pathogen from a diversity of lactose-fermenting bacteria.

Conclusions
e present study revealed a relatively high occurrence of E. coli O157H7. Escherichia coli O157 : H7 isolates developed drug resistance to most antimicrobials tested. All of the E. coli O157 : H7 isolates showed MDR. e study revealed that municipal abattoir and retailer shops in Ambo town did not adhere to the required sanitation and hygiene standards. Proper training and monitoring of meat handlers will help to ensure sanitation and hygienic meat handling practices to provide good quality wholesome meat. e municipal abattoir and retailer shops in the study area should adhere to national and international guidelines.
ere is a need to emphasize the rational use of antimicrobials in agriculture and medicine. In addition, regular antimicrobial susceptibility surveillance is essential. Further research is recommended to validate the source and point of contamination.

Data Availability
All relevant data are included within the paper. e dataset is available from the corresponding author and can be obtained upon reasonable request.
Ethical Approval e protocol of the research project was reviewed and approved by the University of Gondar, School of Biomedical and Laboratory Sciences Ethical Review Committee. Permission to conduct the study was also obtained from the Ambo town municipality.

Consent
Informed written consent was obtained from each study subject before they were asked to give information and meat samples and they were informed that all the information and results of meat samples are only for the purpose of the study.

Disclosure
University of Gondar and Ambo University had no role in the study design, data collection, analysis, and interpretation of the data.

Conflicts of Interest
e authors declare that they have no conflicts of interest.

Authors' Contributions
Nega Desalegn Tadese participated in study design, proposal writing, sample collection, laboratory analysis, data analysis, result interpretation, write-up of the draft, and final versions of the manuscript. Endrias Zewdu Gebremedhi, Belay Tessema, and Feleke Moges contributed to the designing of the study, proposal write-up, result interpretation, and editing. Lencho Megersa Marami, Edilu Jorga Serba, Hirut Abebe, Kebede Abdisa, Dagmawit Atalel, and Bizunesh Mideksa Borana participated in laboratory works and writeup of final versions of the manuscript and editing. All authors contributed to the final version of the manuscript and approved the submission.