Abstract
Background:
Yersinia species, especially Yersinia enterocolitica, are considered as the most prevalent milk-borne pathogens. Several serological and molecular techniques have been developed for rapid and safe diagnosis of yersiniosis.Objectives:
This study was carried out to assess the prevalence rate of Yersinia species, especially Y. enterocolitica, in milk and dairy products in Isfahan province, Iran.Materials and Methods:
A total of 285 commercial and traditional dairy products as well as 267 pasteurized and raw milk samples were collected during one year. The samples were studied by culturing and the positive-culture samples were investigated using PCR techniques.Results:
The results of culture showed that 52 (9.42%) and 28 (5.07%) of the total 552 milk and dairy samples were positive for presences of Yersinia species and Y. enterocolitica, respectively. Totally, 24 of 28 Y. enterocolitica isolates by culture were positive in PCR test (4.59%). Raw cow milk and traditional cheese had the highest prevalence of Yersinia species and Y. enterocolitica, respectively. There were no positive results for pasteurized cow milk, raw camel milk, commercial ice cream, commercial cheese, yoghurt, Doogh, butter and curd. Yersinia species and Y. enterocolitica had the highest prevalence in autumn (15.15% and 10.6%, respectively). Significant differences regarding P < 0.05 were observed between the presences of Yersinia species and Y. enterocolitica in various samples and seasons.Conclusions:
Sanitation and pasteurization are the best ways to increase the microbial quality and particularly decrease the load of Yersinia species. The ability of Yersinia species to growth in Doogh, yoghurt, curd and butter is very low.Keywords
1. Background
Yersinia enterocolitica is a small rod-shaped Gram-negative coccobacillus psychrotrophic enterobacterium, isolated from a variety of environmental sources, foods, and human clinical samples (1-4). It is a causative organism in several outbreaks of gastroenteritis, in which foods were implicated (3, 5). It seems that foods with animal origins have the highest risk of gastrointestinal diseases caused by Y. enterocolitica in humans (1, 2, 6). Milk and dairy products are the most consumed foods with animal origins. In addition, several studies have reported the presence of Y. enterocolitica in milk and dairy products (1, 2, 7-10). Y. enterocolitica has a particular public health importance, because of its capability of growing in raw milk and viability at refrigeration temperatures for long time. Therefore, consumption of milk and dairy products has a higher chance of infection by Y. enterocolitica in humans. Consumption of raw milk and traditional dairy products is common in some areas of Iran; but, the most important issue about Y. enterocolitica is its surveillance in pasteurized milk and even commercial dairy products.
2. Objectives
The dairy-borne issue of Y. enterocolitica is essentially unknown in Iran. Therefore, the present study was carried out to investigate the prevalence of Yersinia species and Y. enterocolitica in raw and pasteurized milk as well as traditional and commercial dairy products in Isfahan province, Iran
3. Materials and Methods
3.1. Samples Collection
From January 2011 to January 2012, a total of 285 diary product samples including commercial cheese (n = 30), traditional cheese (n = 60), commercial ice cream (n = 15), traditional ice cream (n = 35), commercial yoghurt (n = 10), traditional yoghurt (n = 25), commercial Doogh (10), traditional Doogh (20), commercial butter (n = 15), traditional butter (n = 25), commercial curd (15) and traditional curd (35) were purchased from supermarkets and retailers in various parts of Isfahan, Iran. Totally, all of these samples were solid except for commercial and traditional Doogh. All dairy products were kept under refrigeration in plastic bags; information about dates of production and assigned shelf lives was not presented. Besides, 267 milk samples including raw cow milk (n = 80), pasteurized cow milk (n = 30), raw sheep milk (n = 60), raw goat milk (n = 60), and finally raw camel milk (n = 37) were purchased from the same locations. All milk samples showed normal physical characterizations and after collection, they were immediately transferred to the laboratory in a cooler with ice-packs. Samples were collected from various seasons of the year.
3.2. Identification of Yersinia Species
Totally, 25 mL of liquid samples and 25 g of solid samples were aseptically added to 100 mL 0.01 M phosphate buffered saline (PBS, pH 7.6) in a sterile stomacher plastic bag and homogenized for 2 minutes. The homogenates were incubated at 25°C for 10 minutes. Different enrichment procedures were applied. One of the methods was adding 20 mL of the homogenate to 80 mL of trypticase soya broth (TSB) (Oxoid, UK) and enriching the mixture at 25°C for 24 hours. Another procedure was adding 20 mL of the homogenate to 80 mL of PBS and enriching the mixture at 4°C for 14 days (cold enrichment). The samples were treated with KOH (0.5% KOH in 0.5% saline) to suppress the background flora after enrichment. Sub-culturing on selective CIN (cefsulodin-irgasan-novobiocin) agar plates (Yersinia selective agar base, Oxoid UK) was applied according to the method of the FDA (11).
One to the five susceptible colonies of typical “bull’s eye” appearance on the CIN agar plates, if available, were streaked onto tryptone soya agar (Oxoid, UK) plates to create a pure culture. All the isolates from pure cultures were examined for Gram staining, utilization of Simmon’s citrate, motility at 35°C and 27°C, Voges-Proskauer reaction at 35°C and 27°C, Kligler’s iron agar reaction, urease activity, indole production, triple sugar iron butt, slant, nitrate reduction, H2S, lysine decarboxylase, ornithine decarbozylase, oxidase, catalase, dextrose, lactose, sucrose, salicin, maltose, mannitol, rhamnose, arabinose, raffinose, inositoland sorbitol (11) (Table 1).
| Substrate or Test | Reaction | Substrate or Test | Reaction |
|---|---|---|---|
| Gram staining | - | Lysine decarboxylase | - |
| Utilization of Simmon’s citrate | - | Ornithine decarbozylase | + |
| Motility at 35°C | - | Oxidase b | - |
| Motility at 27°C | + | Catalase | + |
| Voges-Proskauer at 35°C | - | Dextrose | A |
| Voges-Proskauer at 27°C | + | Lactose | - |
| Xylose | A | Sucrose | A |
| Urease activity | + | Salicin | - |
| Indole production | + | Maltose | A (delayed) |
| Triple sugar iron butt | A | Mannitol | A |
| Slant | A | Rhamnose | - |
| Nitrate reduction | + | Arabinose | A |
| H2S | - | Raffinose | - |
| Sorbitol | A | Inositol | A (delayed) |
3.3. DNA Extraction and Polymerase Chain Reaction
The bacterial strains which were cultivated on CIN medium and biochemically identified as Y. enterocolitica, were confirmed using the PCR method. Purification of DNA from bacterial colonies was achieved using a genomic DNA purification kit (Fermentas, Germany) according to the manufacturer’s instructions. To specifically amplify the Y. enterocolitica 16S rRNA gene, a set of primers, Y1 (5’-AATACCGCATAACGTCTTCG-3’) and Y2 (5’-CTTCTTCTGCGAGTAACGTC-3’), was used, resulting in a PCR product of 330 bp (12). The PCR products were stained with 1% solution of ethidium bromide and visualized under the UV light after electrophoresis on 1.5% agarose gel.
3.4. Statistical Analysis
Differences in the prevalence of Yersinia spp. and Y. enterocolitica in various milk and dairy products were analyzed using a chi-square test in SPSS for Windows (release 18.0 standard version, SPSS Inc., Chicago, Illinois). The differences were considered statistically significant when P < 0.05.
4. Results
Results of the present study confirmed the presence of Yersinia spp. and especially Y. enterocolitica in milk and dairy products. The culture method showed that from a total of 552 milk and dairy samples, 52 (9.42%) were positive for presences of Yersinia spp. (Table 2). After biochemical analysis of positive samples, it was recognized that from a total of 552 samples, 28 (5.07%) were positive for Y. enterocolitica (Table 2). On the other hand, from a total of 52 Yersinia spp. isolates, 28 (53.84%) were Y. enterocolitica. Our results showed that raw cow milk (16.25%) and traditional cheese (23.33%) had the highest prevalence of Yersinia spp. and Y. enterocolitica among milks and dairy products, respectively (Table 2). Results showed that there were no bacteria in pasteurized cow milk, raw camel milk, commercial cheese, commercial ice cream and both types of yoghurt, Doogh, butter and curd (Table 2). After PCR, it was recognized that from a total of 552 samples, 24 (4.34%) were positive for Y. enterocolitica 16 srRNA gene (Table 2).
Table 3 shows the distribution of Yersinia spp. and Y. enterocolitica in dairy samples in various seasons. Autumn had the highest (15.15% and 10.6%) while summer had the lowest (5.71% and 2.14%) prevalence of Yersinia spp. and Y. enterocolitica, respectively.
Prevalence of Yersinia spp. and Y. enterocolitica in Milk and Dairy Products in Iran Using Culture and PCR Method a
| Type of Food | Number of Samples | Culture Method | PCR Method | |
|---|---|---|---|---|
| Yersinia spp. | Y. enterocolitica | Y. enterocolitica | ||
| Raw cow milk | 80 | 13 (16.25) b | 8 (10) b | 6 (7.5) b |
| Pasteurized cow milk | 30 | - | - | - |
| Raw sheep milk | 60 | 5 (8.33) | 3 (5) | 3 (5) |
| Raw goat milk | 60 | 2 (3.33) | 1 (1.66) | 1 (1.66) |
| Raw camel milk | 37 | -b | -b | -b |
| Cheese | 90 | 14 (15.55)c | 7 (7.77)c | 6 (6.66)c |
| Commercial cheese | 30 | -b | -b | -b |
| Traditional cheesed | 60 | 14 (23.33) | 7 (11.66) | 6 (10) |
| Ice cream | 50 | 2 (4) | 1 (2) | 1 (2) |
| Commercial ice cream | 15 | -b | -b | -b |
| Traditional ice cream | 35 | 2 (5.71)b | 1 (2.85)b | 1 (2.85)b |
| Yogurt | 35 | - | - | - |
| Commercial yogurt | 10 | - | - | - |
| Traditional yogurt | 25 | - | - | - |
| Dooghc | 30 | - | - | - |
| Commercial Doogh | 10 | - | - | - |
| Traditional Doogh | 20 | - | - | - |
| Butter | 40 | - | - | - |
| Commercial butter | 15 | - | - | - |
| Traditional butter | 25 | - | - | - |
| curd e | 50 | - | - | - |
| Commercial curd | 15 | - | - | - |
| Traditional curd | 35 | - | - | - |
| Total | 552 | 52 (9.42) | 28 (5.07) | 24(4.34) |
5. Discussion
Milk is raised as a complete food, especially for children and seniors. Its high values of proteins, minerals, fats and vitamins are undeniable. It is the primary source of nutrition for young mammals before they are able to digest other types of foods. In addition, milk has been transformed into various dairy products such as cheese, cream, butter, yogurt, kefir, Doogh, curd and ice cream. In a day, millions of people use milk and dairy products. Therefore, hygienic quality of milk and dairy products is very important; but sometimes it decreases, causing several infections and illness.
Foodborne diseases are among worldwide growing health problems, including a wide spectrum of illnesses caused by microbial, viral, parasitic or chemical contamination of food. Previous reports showed that among all foodborne pathogens such as Y. enterocolitica, Clostridium botulinum, Campylobacter jejuni, Escherichia coli O157:H7, Listeria monocytogenes, Salmonella spp., Shigella spp. and Bacillus cereus, the first one is the most common foodborne bacterium in foods with animal origins (6, 13, 14). As far as we know, several investigations have reported outbreaks of foodborne infections caused by Y. enterocolitica, in which contaminated milk was incriminated (15, 16).
To our knowledge, such surprisingly high percentage of positive results (9.42%) had never been reported in Iran. Only one study has been conducted on detection of Y. enterocolitica in milk in Iran. This study showed that five samples (1.6%) of raw milk, but no pasteurized milk samples, were positive for Y. enterocolitica (1), which was lower than our results. Another study in Iran showed that 15.8% of meat and chicken samples were contaminated with Y. enterocolitica (17). Our study showed significant differences (P < 0.05) in the presences of Yersinia spp. and Y. enterocolitica, in comparison of raw cow milk with pasteurized cow milk and raw camel milk. Furthermore, there were significant differences in the presences of Yersinia spp. and Y. enterocolitica, comparing traditional cheese with commercial cheese and traditional ice cream with commercial ice cream (P < 0.05). It seemed that there was no significant difference in confidence level of 95% between the ability of culture with PCR technique for detection of Yersinia spp. and Y. enterocolitica.
In a study in Morocco, Yersinia spp. was recovered from 11 of 30 raw milks (36.6%), 1 of 20 pasteurized milks (5%), 15 of 63 traditional fermented milks (23.8%), 7 of 94 cheeses (7.44%), and 1 of 20 cream samples (5%), and the overall incidence of Y. enterocolitica in milk and dairy products was 6.6% (18), which was slightly higher than our results (5.07%). Another study showed that the prevalence of Y. enterocolitica was 24.1% in raw buffalo milk; however, no isolation could be made from the pasteurized milk samples (19) and this was in agreement with our research. Our study was the first prevalence reports of Yersinia spp. and Y. enterocolitica in camel milk, Doogh, curd, butter and yoghurt samples in Iran. In our study, there were no positive results for presences of Yersinia spp. and Y. enterocolitica in the above samples. Therefore, there was no possibility for the presence of Yersinia spp. and Y. enterocolitica in the pasteurized milk and camel milk. In despite of these two types of samples, other types of dairy products can be reservoir for Yersinia spp.
Curd is a dairy product prepared by prolonged boiling of yogurt. Doogh is a dairy product prepared by beating unflavored yogurt until smooth, and then diluting with water to a consistency similar to whole milk; it is also called yogurt soda. Different pH values have the golden role in the prevalence of Y. enterocolitica in different samples. Bhaduri et al. (20) reported no development of Y. enterocolitica at pH = 4.5 and low temperatures (5°C to 19°C). Brackett (21) found that this bacterium remained viable at pH = 4 for at least 21 days at 5°C. The Y. enterocolitica isolated from milk and dairy samples of our study, was recovered from samples with pH of 4.8-5 at 4°C. Probably, curd, Doogh and yoghurt, studied in our research, had high activated water. Therefore, these samples had high acidity and there were no possibility for their bacterial contamination.
Old studies conducted on raw milk in Alsace and France showed that out of 75 tested samples, 61 (81.4%) were contaminated with Yersinia spp. (22). An Irish study showed that 279 of 589 dairy samples were contaminated with Yersinia spp., 59% of which were Y. enterocolitica (23), which was higher than our results (53.84%). A Turkish study performed on 211 raw milk samples, revealed 33 pathogenic microorganisms, among which eight were Y. enterocolitica (24). A study in Pennsylvania showed a lower amount of bulk tank milk contamination with Y. enterocolitica (1.2%) (10).
Our results showed that traditional ice creams were one of the main sources of Y. enterocolitica (2.85% prevalence rate). In a previous study, Y. enterocolitica was isolated from samples of ingredients used in the production of ice cream, such as cream, egg, and pasteurized milk (16). Furthermore, several studies have reported isolation of Y. enterocolitica from ice cream (25, 26).
A previous study showed that the occurrence of Y. enterocolitica was slightly higher in processed milk (73.8% positive) than bulk tank milk (64.7%) (22) and this was in contrast with our results. A study in USA (14) showed that from a total of 292 bulk tank milk samples, 4.1%, 12.1%, 15.1% and 8.9% of samples were positive for L. monocytogenes, C. jejuni, Y. enterocolitica and salmonella, respectively. Therefore, Y. enterocolitica had the highest prevalence among milk-borne pathogens. In a study in Dakota, C. jejuni, shiga-toxin producing E. coli, L. monocytogenes, Salmonella spp. and Y. enterocolitica were detected in 9.2%, 3.8%, 4.6%, 6.1%, and 6.1% of bulk tank milk samples, respectively (10).
In a study in Turkey, from a total of 100 white cheese samples purchased from retailers, supermarkets and factories, 8 (8%) were positive for presence of Y. enterocolitica using the culture method (27), which was in agreement with our study. Another study in Turkey showed that from a total of 14 and 55 Yersinia spp. isolates, respectively isolated from raw milk and traditional cheese with pH of 4-5, 7.1% were Y. intermedia,47.3% Y. enterocolitica, 31% Y. fredriksen, 7.2% Y. intermedia, 12.7% Y. Christensen and finally 1.8% were other species of Yersinia (28).
Our results showed that the prevalence of Yersinia spp. and Y. enterocolitica in milk and dairy products had a seasonal pattern. These bacteria had the highest prevalence in autumn and the lowest in winter. Statistical analysis showed significant differences in the presence of Yersinia spp. and Y. enterocolitica between milk and dairy samples of autumn and summer (P < 0.05). Another study showed that the incidence of Y. enterocolitica in milk and dairy products were much higher (25-50%) during winter compared with summer (0-17%) (19). Seasonal prevalence of this bacterium was previously reported (29-32), in all of which the prevalence of Y. enterocolitica was higher in warmer seasons.
Rare cases of mastitis have been associated with Yersinia spp. in Israel (33). More commonly, risk factors for contamination of raw milk are likely to be those associated with poor hygiene of milking and fecal contamination of the teat ends prior to milking cup attachment. The differences between findings of various authors and those of this study might be due to several factors such as method of sampling, number of analyzed samples, method of analyzing, sources of samples, season, and geographical location. These factors may cause an increase or decrease in the incidence of Yersinia spp. infection. Neither vaccines for prevention of yersiniosis in animals nor any routinely available tests for subclinical infections are currently available. Control of this pathogen relies on effective hygiene management of the farm, especially the milking practice.
Our results showed that using raw milk without pasteurization, milking with unsanitary methods, and using traditional dairy products produced in unsanitary conditions and probably from unpasteurized milk, are the main resources for growth, proliferation and survival of Y. enterocolitica. These factors cause several disorders for human. Therefore, improving the methods of milking, monthly checking of the milking halls to detect Y. enterocolitica especially in the animal feces, fumigating the milking halls frequently, inspecting the hygiene during milking, boiling the milk, using pasteurized and even sterilized milk for dairy products, keeping dairy products in cool and dry places away from the sunlight, and finally preventing from contamination of dairy products with extrinsic factors such as insects and dust, are the best ways to prevent Y. enterocolitica infections.
Acknowledgements
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