Epidemiology and Molecular Prevalence of Toxoplasma gondii in Cattle Slaughtered in Zahedan and Zabol Districts, South East of Iran

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Iran J Parasitol: Vol. 13, No. 1, Jan-Mar 2018, pp.114-119 Iran J Parasitol Tehran University of Medical Sciences Publication http://tums.ac.ir Open access Journal at http://ijpa.tums.ac.ir Iranian Society of Parasitology http://isp.tums.ac.ir Short Communication Epidemiology and Molecular Prevalence of Toxoplasma gondii in Cattle Slaughtered in Zahedan and Zabol Districts, South East of Iran Davood ANVARI 1, *Dariush SAADATI 2, Reza NABAVI 3, Majid ALIPOUR ESKANDANI 2 1. Faculty of Veterinary Medicine, University of Zabol, Zabol, Iran 2. Dept. of Nutrition and Animal Breeding, Faculty of Veterinary Medicine, University of Zabol, Zabol, Iran 3. Dept. of Pathobiology, Faculty of Veterinary Medicine, University of Zabol, Zabol, Iran Received 26 Feb 2017 Accepted 14 Sep 2017 Keywords: Toxoplasma, Cattle, PCR, Iran *Correspondence Email: saadatidariush@yahoo.com Abstract Background: Toxoplasma gondii is an obligate, intracellular parasite which causes the toxoplasmosis in humans and warm-blooded animals. Red meat is an important source for transmission of the infection to humans. This study aimed to determine the prevalence of Toxoplasma among imported and indigenous cattle in the Sistan region. Methods: One hundred samples from slaughtered cattle were collected from two abattoirs of Zabol and Zahedan, South East of Iran in 2015. Each sample was a mixture of three muscle, including tongue, cardiac, and triceps. Additional data of each cattle, including sex, breed, age, indigenous or imported, location of slaughter, management practices, and feeding system were obtained through observations and interviews. Infection by T. gondii was determined by PCR method. Results: The prevalence of Toxoplasma in indigenous cattle was 6% and in imported cattle was 26%, and this difference was statistically significant (P=0.006). Moreover, the prevalence of Toxoplasma was statistically associated with management practices (P=0.01) and feeding system (P=0.001). However, relationship between the prevalence of Toxoplasma with age, breed, sex, and location of slaughter was not statistically significant. Conclusion: Since the prevalence of Toxoplasma among imported cattle is higher than indigenous cattle, so strict supervision for importing livestock from neighboring countries is necessary. 114 Available at: http://ijpa.tums.ac.ir

Anvari et al.: Epidemiology and Molecular Prevalence of Toxoplasma gondii Introduction T oxoplasma gondii is a protozoan parasite that is spread around the world. Although Toxoplasmosis in human often occur asymptomatically, when the infection is transmitted congenitally, and in immunocompromised patients, it can cause severe symptoms (1). Cat is the definitive host of T. gondii and all warm-blooded animals, including humans are intermediate hosts. Definitive host in the early stages of infection excretes several millions of resistant oocysts (2). The oocysts sporulation period is 1-5 d in the natural environmental condition. The infection of intermediate host occurs after ingesting of sporulated oocyst from soil, water or plants (3). Shortly after ingestion, tachyzoites move to be localizing in muscles and nervous system. Finally, the tissue cysts develop including some bradyzoites (3). Humans can be infected either by eating food and water containing infected oocyst or by eating meat containing bradyzoites and tachyzoites (2). Natural infection of cattle with T. gondii will not cause clinical symptoms and abortion (4). However, beef plays a special role in epidemiology of toxoplasmosis. Because in some cases beef is consumed as grilled and undercooked, so it is important for the transmission of Toxoplasma to humans. Because the lack of apparent complications on contaminated carcasses, detect of toxoplasmosis in the slaughterhouse during visual inspection is not possible. Various laboratory methods for the detection of toxoplasmosis are used. Molecular methods such as polymerase chain reaction (PCR) assay offer advantages of remarkable sensitivity, high specificity, and speed in diagnosis (5). In the recent years, a large number of imported cattle are slaughtered in Sistan and Baluchestan Province and there is not any information about prevalence of Toxoplasma in these animals. Therefore, this study determined the prevalence of Toxoplasma among imported and indigenous cattle in the Sistan region. Materials and Methods One hundred cattle carcasses in two abattoirs of Zabol (50 carcasses) and Zahedan (50 carcasses), South East of Iran were sampled in 2015. In any abattoir, half of the samples (25 cases) were indigenous cattle and the others (25 cases) were imported cattle from Pakistan. The samples were taken from each abattoir in three times. In the first, second and third time respectively 16, 16 and 18 carcasses were sampled. Sampling in slaughter line was performed using systematic random sampling method. Additional data of each cattle, including sex, breed, age, indigenous or imported, location of slaughter, management practices, and feeding system were obtained through observations and interviews. Cattle were placed in two categories based on the management practice of the farm to which they belonged. In industrial management, animals are kept at high stocking densities, with large amounts of meat or milk production. These farms are usually far away from residential areas. However, in traditional management, animals are kept in a stable in beside of farmer's house. This farming system is common in rural areas. PCR Procedure Three samples from each carcass, including the tongue, heart, and triceps were taken. The volume of each sample was one cubic centimeter (approximately one gram). The samples were minced by sterile scalpel and the mixture was poured into a sterile Eppendorf tube. Containing each Eppendorf was used following the manufacturer s instructions of a commercial DNA extraction kit (MBST, Iran) the samples were suspended in 180µL Lysis Buffer and 20 µl proteinase K. Then 360 µl binding buffer was added to each tube and the protocol recommended for tissue samples was followed. All DNA extracts were stored at -20 ºC for use in PCR reaction. Available at: http://ijpa.tums.ac.ir 115

Iran J Parasitol: Vol. 13, No. 1, Jan-Mar 2018, pp.114-119 The primers TOX4 (5'CGCTGCAGGGAGGAA- GACGAAAGTTG3') and TOX5 (5'CGCTGCAGA- CACAGTGCATCTGGATT3') were selected for PCR assay. These primers amplified a noncoding 529 bp fragment that is repeated 200-300-fold in the genome of T. gondii (6). The reaction conditions were as follows: one initial denaturation cycle for 7 min at 94 ºC, 40 cycles of denaturation at 94 ºC for 45 sec, annealing at 55 ºC for 45 sec, and extension at 72 ºC for 45 sec. The procedure was completed by a final cycle extension for 7 min. The positive control was obtained from Parasitology Department, Shahid Beheshti University of medical science. Samples without genomic DNA were included as negative controls. The PCR products were analyzed on 2% agarose gel and stained using ethidium bromide and visualized in the UV illuminator (Fig. 1). Statistical Methods Association between infection with T. gondii (the dependent variable) and independent variables was investigated using Chi-square test and Fisher exact test. SPSS ver. 18 (Chicago, IL, USA) was used for statistical analysis. Fig. 1: Amplified a non-coding 529 bp fragment for Toxoplasma gondii. P is positive control and N represents the negative control, and M is 100 bp marker. Moreover, 1 to 6 is some positive samples. Results From 50 samples of indigenous cattle, 3 (6 %) and from 50 samples of imported cattle, 13 (26 %) were shown to be positive by PCR method. The Pearson s Chi-squared test showed that the observed difference between indigenous cattle and imported cattle is statistically significant. Moreover, traditional livestock and pasture feeding significantly increase the risk of occurrence of toxoplasmosis. However, effects of location of slaughter, breed, sex, and age on prevalence of T. gondii are not statistically significant (Table 1). 116 Available at: http://ijpa.tums.ac.ir

Anvari et al.: Epidemiology and Molecular Prevalence of Toxoplasma gondii Table 1: the distribution of Toxoplasma prevalence based on PCR according to city, location of livestock, type of livestock, feeding, sex, breed, and age Category Levels No. of tested No. of positive Prevalence P-Value animals animals (%) Location of slaughter Zabol 50 6 12.0 0.275 Zahedan 50 10 20.0 Location of livestock Indigenous 50 3 6.0 0.006 Imported 50 13 26.0 Management practices Industrial 26 0 0.0 0.01 Traditional 74 16 21.6 Feeding Pasture 30 11 36.7 0.001 Manual 70 5 7.1 Sex Female 3 0 0.0 0.589 Male 97 16 16.5 Breed Holstein 61 13 21.3 0.070 Sistani 39 3 7.7 Age Upper 2 year 85 15 17.6 0.259 Under 2 year 15 1 6.7 Discussion In this research, the overall prevalence of Toxoplasma infection in slaughtered cattle meat was estimated 16.0%. In Ahvaz (Iran), samples of tongue, heart, and muscle were taken from lamb and beef and meat product samples (sausages, hamburgers, and salami) and PCR used for detection of T. gondii (7). The overall prevalence of Toxoplasmosis was 14% in lambs, 4% in beef and 0% in meat product samples. The prevalence of Toxoplasma in cattle, camels and sheep in the provinces of Isfahan and Chaharmahal and Bakhtiari (Iran) was evaluated using the PCR method (8) that T. gondii infections were detected in 0.0%, 6.6% and 17.9% of the samples of cattle (n = 155), camels (n = 122) and sheep (n = 95), respectively. In Lorestan Province (Iran), 174 serums of Cattle were collected from the slaughterhouses, the serum samples were examined via Indirect Immunofluorescence antibody test, and the IgG prevalence rate was 28.73% (9). Among livestock referred to surgery Department of Veterinarian College in Urmia University (Iran), the seroprevalence of Toxoplasma gondii in cattle, sheep, and horses were 1.6%, 21.1% and 11.5% (10). In addition, a systematic review and meta-analysis was conducted on the occurrence of toxoplasmosis in cattle in Iran (11). Pooled proportion of toxoplasmosis, among cattle in Iran from 1983 to 2012 was 18.1% (95% CI: 9.9% to 28.2%). seropositive rate of cattle toxoplasmosis in various regions of Iran was between 1.4% and 71.3% in Kerman and Tehran Province (11). Toxoplasmosis was endemic in livestock in the most parts of the country including Sistan region and this is important in terms of the public's health. Prices of livestock in the eastern neighboring countries are cheaper than Iran. Therefore, in the recent years, a large number of Cattle have been imported from these countries to Sistan and Baluchistan Province. In the present study, the prevalence of T. gondii in imported cattle from Pakistan was significantly more than indigenous cattle. In South-West Pakistan, the seroprevalence of Toxoplasma gondii infections among 100 cattle was measured by using latex agglutination test (LAT). Positive titers for Toxoplasma were detected in 25% of cattle (12). In Punjab Province (Pakistan), 200 serum samples of cattle were examined for the detecting of T. gondii by using Latex Agglutination Test (LAT). Overall, 87 cat- Available at: http://ijpa.tums.ac.ir 117

Iran J Parasitol: Vol. 13, No. 1, Jan-Mar 2018, pp.114-119 tle (43.5%) were seropositive (13). In private and government-owned farms in Punjab Province (Pakistan), serum samples were taken from 400 cattle. The samples were tested using enzyme-linked immunosorbent assay (ELISA). The overall prevalence of infection was 19.75% (79/400). Moreover, IgG and IgM antibodies were found in 75 cattle (18.75%), and 9 cattle (2.25%) respectively (14). Toxoplasma was hyperendemic among Pakistani cattle. The prevalence of Toxoplasma in cattle was associated with feeding system. Cattle graze in the pasture than those fed manually are more likely to become contaminated with sporulated oocysts. In Lorestan Province (Iran), the prevalence of T. gondii in cattle was lower than sheep and goats (29% vs 53% and 52%). Cattle were often fed manually, but sheep and goats graze in pastures (9). The prevalence of Toxoplasma in industrial livestock was significantly less than traditional livestock and stray cats roaming mostly on traditional farms. They can contaminate water and forage in their feces. A significant association was found between prevalence of Toxoplasma and exposure of cattle to cats. Including a study on risk factors of toxoplasmosis in large ruminants showed that presence of cats in the surrounding areas of cattle is an important risk factor for infection of cattle (14). In addition, in Brazil, seroprevalence of T. gondii in cattle was depended on number of cats in farm, contact of cats with cattle and contact of cat with drinking water (15). Besides, Proper hygiene in industrial farms is due to the less occurrence of toxoplasmosis in this livestock. In addition, in this study, all cattle reared industrially, were feeding manually, and the low prevalence of Toxoplasma in such industrial group is related to feeding pattern. Similar findings in sheep have also been reported in Zimbabwe. Toxoplasmosis in Sheep from commercial farms was significantly lower than that of Sheep from the communal grazing system (16). In the present study, the prevalence of infection was not statistically associated with location of slaughter, age, breed, and gender of cattle. The prevalence of this parasite in female cattle was statistically more than male animals (17), as well as female animals, were more susceptible than males for toxoplasmosis (18). However, in Tabriz (Iran), antibody to Toxoplasma in male cattle was significantly more than females (19). Conclusion The prevalence of Toxoplasma gondii in the meat of imported cattle from Pakistan is higher than indigenous livestock. Since the Toxoplasma endangers human health, meat of imported cattle could be freeze before offering to market for decreasing of occurrence of toxoplasmosis in humans. Moreover, strict supervision for importing livestock from neighboring countries is necessary. Acknowledgments This work was financially supported by Vic chancellor for research and technology, University of Zabol, Iran (Number financing agreement: 93-5). Conflict of interest The authors declare that there is no conflict of interest. References 1. Daryani A, Sarvi S, Aarabi M et al. Seroprevalence of Toxoplasma gondii in the Iranian general population: A systematic review and meta-analysis. Acta Trop. 2014; 137:185-194. 2. Opsteegh M, Langelaar M, Sprong H et al. Direct detection and genotyping of Toxoplasma gondii in meat samples using magnetic capture and PCR. Int J Food Microbiol. 2010;139(3):193-201. 118 Available at: http://ijpa.tums.ac.ir

Anvari et al.: Epidemiology and Molecular Prevalence of Toxoplasma gondii 3. Motarjemi Y, Moy G, Todd E. Encyclopedia of food safety. Amsterdam: Academic Press; 2014. 4. Dubey J. A review of toxoplasmosis in cattle. Vet Parasitol. 1986; 22(3-4):177-202. 5. MacPherson JM, Gajadhar AA. Sensitive and specific polymerase chain reaction detection of Toxoplasma gondii for veterinary and medical diagnosis. Can J Vet Res. 1993;57(1):45-8. 6. Homan W, Vercammen M, De Braekeleer J, Verschueren H. Identification of a 200-to 300- fold repetitive 529 bp DNA fragment in Toxoplasma gondii, and its use for diagnostic and quantitative PCR. Int J Parasitol. 2000; 30(1):69-75. 7. Rahdar, M., A. Samarbaf-Zadeh, and L. Arab. Evaluating the prevalence of Toxoplasma gondii in meat and meat products in Ahvaz by PCR method. Jundishapur J Microbiol. 2012; 5(4):570-3. 8. Khamesipour F, Doosti A, Mobarakeh HI, Komba EV. Toxoplasma gondii in Cattle, Camels and Sheep in Isfahan and Chaharmahal va Bakhtiary Provinces, Iran. Jundishapur J Microbiol. 2014; 7(6): e17460. 9. Hashemi S. Seroprevalence of toxoplasmosis in cattle, sheep and goat, using ELISA and Indirect Immunoflorescent Antibody (IFA) methods in Lorestan province. Journal of Large Animal Clinical Science Research. 2014; 7(2):49-55. 10. Raeghi S, Akaberi A, Sedeghi S. Seroprevalence of Toxoplasma gondii in sheep, cattle and horses in Urmia North-West of Iran. Iran J Parasitol. 2011; 6(4):90-94. 11. Sarvi S, Daryani A, Rahimi MT et al. Cattle toxoplasmosis in Iran: a systematic review and meta analysis. Asian Pac J Trop Med. 2015; 8(2):120-126. 12. Zaki M. Seroprevalence of Toxoplasma gondii in domestic animals in Pakistan. J Pak Med Assoc. 1995; 45(1):4-5. 13. Zahida T, Zunera S, Mushtaq HL, Fariha A. Seroprevalence of Toxoplasma gondii in Cattle, Punjab, Pakistan. Glob Vet. 2013; 11(5):681-684. 14. Ahmad N, Qayyum M. Seroprevalence and risk factors for toxoplasmosis in large ruminants in northern Punjab, Pakistan. J Infect Dev Ctries. 2014; 8(8):1022-8. 15. Albuquerque GR, Munhoz AD, Teixeira M et al. Risk factors associated with Toxoplasma gondii infection in dairy cattle, State of Rio de Janeiro. Pesq Vet Bras. 2011; 31(4):287-290. 16. Hove T, P Lind, S Mukaratirwa. Seroprevalence of Toxoplasma gondii infection in goats and sheep in Zimbabwe. Onderstepoort J Vet Res. 2005; 72(4):267-272. 17. Asgari Q, Sarnevesht J, Kalantari M et al. Molecular survey of Toxoplasma infection in sheep and goat from Fars province, Southern Iran. Trop Anim Health Prod. 2011; 43(2):389-392. 18. Alexander J, Stimson WH. Sex hormones and the course of parasitic infection. Parasitol Today. 1988; 4(7):189-193. 19. Nematollahi A, Moghddam G. Survey on seroprevalence of anti-toxoplasma gondii antibodies in cattle in Tabriz (Iran) by IFAT. Am J Anim Vet Sci. 2008; 3(1):40-42. Available at: http://ijpa.tums.ac.ir 119