Inpankaew_161-165.indd INTRODUCTION Cryptosporidium parvum is an obligate intracellular protozoan parasite that mainly infects the gastro- intestinal tract of a wide range of vertebrates includ- ing livestock and humans (Current & Garcia 1991). Infection of immunocompetent humans can induce acute, self-limiting diarrhoea. In contrast, infection of immunodeficient individuals frequently results in persistent, severe and life-threatening diarrhoea (Gu errant 1997). Cryptosporidium parvum is the most frequent parasitic agent that causes diarrhoea in AIDS patients in Thailand. Moreover, Manatsathit, Tansupasawas dikul, Wanachiwanawin, Setawarin, Su wanagool, Pra kas vejakit, Leelakusolwong, Eam- pokalap & Kach intorn (1996) reported that C. par- vum is the most common enteric pathogen contrib- 161 Onderstepoort Journal of Veterinary Research, 76:161–165 (2009) Seroprevalence of Cryptosporidium parvum infection of dairy cows in three northern provinces of Thailand determined by enzyme-linked immunosorbent assay using recombinant antigen CpP23 T. INPANKAEW1, 3, S. JITTAPALAPONG1, J. PHASUK1, N. PINYOPANUWUT1, W. CHIMNOI1, C. KENGRADOMKIT1, C. SUNANTA2, G. ZHANG3, G.O. ABOGE3, Y. NISHIKAWA3, I. IGARASHI3 and X. XUAN3* ABSTRACT INPANKAEW, T., JITTAPALAPONG, S., PHASUK, J., PINYOPANUWUT, N., CHIMNOI, W., KEN- GRA DOMKIT, C., SUNANTA, C., ZHANG, G., ABOGE, G.O., NISHIKAWA, Y., IGARASHI, I. & XU- AN, X. 2009. Seroprevalence of Cryptosporidium parvum infection of dairy cows in three northern provinces of Thailand determined by enzyme-linked immunosorbent assay using recombinant anti- gen CpP23. Onderstepoort Journal of Veterinary Research, 76:161–165 Cryptosporidium parvum is the most frequent parasitic agent that causes diarrhoea in AIDS patients in Thailand. Cryptosporidiosis outbreaks in humans may be attributed to contamination of their drink- ing water from infected dairy pastures. A 23-kDa glycoprotein of C. parvum (CpP23) is a sporozoite surface protein that is geographically conserved among C. parvum isolates. This glycoprotein is a potentially useful candidate antigen for the diagnosis of cryptosporidiosis by enzyme-linked immuno- sorbent assay. Therefore, we investigated the seroprevalence of C. parvum infection in dairy cows in northern Thailand using an ELISA based on recombinant CpP23 antigen. Sera were randomly col- lected from 642 dairy cows of 42 small-holder farmers, which had the top three highest number of the dairy cows’ population in Northern Thailand, that included Chiang Mai, Chiang Rai and Lumpang provinces. The overall seroprevalence of the infection was 4.4 %, and the seropositive rates for the three provinces were 3.3 % in Chiang Mai, 5.1 % in Chiang Rai and 3 % in Lumpang. These results suggest that cattle could play a role in zoonotic cryptosporidiosis in Thailand. Keywords: Cryptosporidium parvum, CpP23, dairy cow, ELISA, Thailand * Author to whom correspondence is to be directed. E-mail: gen@obihiro.ac.jp 1 Department of Parasitology, Faculty of Veterinary Medicine, Kasetsart University, Bangkok, Thailand 2 Chiang Rai Provincial Office, Department of Livestock Devel- op ment, Chiang Rai, Thailand 3 National Research Center for Protozoan Diseases, Obihiro University of Agriculture and Veterinary Medicine, Inada-cho, Obihiro, Hokkaido 080-8555, Japan Accepted for publication 14 August 2008—Editor 162 Cryptosporidium parvum infection of dairy cows in Thailand uting to 20 % of the causes of chronic diarrhoea in AIDS patients in Thailand. In the developing world, Cryptosporidium constitutes part of a complex group of parasitic, bacterial and viral diseases that leads to an inability of infected individuals to achieve their full potential. This com- plex group of infections classified by the World Health Organization (WHO) as “neglected diseas- es”, initiate common diseases associated with pov- erty (Savioli, Smith & Thompson 2006). Crypto spor- idiosis outbreaks in humans are thought to be due to contamination of their drinking water from infect- ed dairy pastures. In a recent survey in the Nong pho dairy region of central Thailand using Cryptosporidium-specific an- tigen (CSA) it was found that the seroprevalence rate of Cryptosporidium infection in dairy cows was 9.4 % (Jittapalapong, Pinyopanuwat, Chimnoi, Siri- panth & Stich 2006). This finding suggested that the infection could also be endemic in other areas in Thailand where the same study had not been done. Hence, there was need for a further investigation into the distribution of cryptosporidiosis in cattle in these regions. Furthermore, the diagnosis of C. parvum infection relies almost exclusively on the microscopic detec- tion of oocysts in faeces, but this method is rela- tively time consuming, subjective and unreliable especially when oocysts shedding in the faeces has ceased. Nevertheless, a serological test based on ELISA is capable of partially fulfilling diagnostic re- quirements because serum antibodies against the parasite persist even after oocysts shedding in fae- ces has ceased. A 23-kDa glycoprotein of C. parvum (CpP23) is a sporozoite surface protein that is geographically conserved among C. parvum isolates. This con- served glycoprotein is potentially a useful candidate antigen for the diagnosis of cryptosporidiosis by ELISA since it is likely to detect C. parvum strains in various geographical regions (Perryman, Kapil, Jones & Hunt 1999). Therefore, an ELISA based on the recombinant CpP23 antigen was used in this study to investigate the prevalence of C. parvum in- fection in dairy cows in the northern part of Thailand. MATERIALS AND METHODS Parasite Cryptosporidium parvum isolate (HNJ-1 strain) was used in this study (Abe, Kimata & Iseki 2002). Cloning of CpP23 gene Purified C. parvum oocysts were lyzed in 0.1 M Tris- HCl (pH 8.0) containing 1 % sodium dodecyl sul- phate (SDS), 0.1 M NaCl, and 10 mM EDTA and then treated with proteinase K (100 μg/mℓ) at 55 °C for 2 h. The genomic DNA pellets were extracted with phenol/chloroform followed by ethanol precipitation. The DNA pellets were dissolved in a TE buffer (10 mM Tris-HCl, pH 8.0, and 1 mM EDTA) and used as a template DNA for PCR. The truncated CpP23 gene without sequences encoding a hydrophobic signal peptide and a C-terminus was amplified by PCR using oligonucleotide primers, 5’-ACGGAT- CCAAAAATGGGTTGTT-3’ and 5’-ACGGATCCT- AATTTAGGCATCA-3’, both containing BamHI sites introduced to facilitate cloning. The PCR product was digested with BamHI and then cloned into the BamHI site of the bacterial expression vector, pGEX-4T-3 (Promega, USA). The resulting plasmid was designated as pGEX/CpP23. Expression of the CpP23 gene in Escherichia coli The recombinant CpP23 gene was expressed as a glutathione S-transferase (GST)-fusion protein (GST-CpP23) in JM109 E. coli (Promega, USA) as described by Takashima, Xuan, Kimata, Iseki, Ko- dama, Nagane, Nagasawa, Matsumoto, Mikami & Otsuka 2003 and then purified. ELISA The ELISA was performed as reported by Bannai, Nishigawa, Seo, Nakamura, Zhang, Kimata, Ta ka- shima, Li, Igarashi & Xuan 2006. Briefly, the purified GST-CpP23 was diluted to an optimal concentra- tion (5 μg/mℓ) in a 50 mM carbonate-bicarbonate buffer (pH 9.6), of which 50 μℓ were added sepa- rately to duplicate wells for each sample. Coated plates were incubated at 4 °C overnight. After the unabsorbed antigen was discarded, the wells were blocked with PBS containing 3 % skim milk (block- ing solution, 100 μℓ per well) at 37 °C for 1 h. The plates were then washed once with PBS containing 0.05 % Tween 20 (PBS-T). Fifty microlitres of serum diluted in the blocking solution (1:100) were added to each well and incubated at 37 °C for 1 h. After incubation, the wells were washed six times with PBS-T and subsequently incubated with 50 μℓ of goat anti-bovine IgG-horseradish peroxidase conju- gate (ICN Biochemical, USA) (1:4 000) at 37 °C for 1 h. After six washes, 100 μℓ of substrate solution [0.05 % 2,2’-azino-bis (3-ethylbenz-thiazoline-6-sul- 163 T. INPANKAEW et al. phonic), 0.2 M sodium phosphate, 0.1 M citric acid, 0.003 % H2O2] were added to each well. After 1 h reaction at room temperature, the optimal density (OD) was read at 415 nm by using an MTP-120 ELISA reader (Corona Electric, Japan). The ELISA titre was expressed as the reciprocal of the maxi- mum dilution that showed an ELISA value equal to or greater than 0.1, which is the difference in ab- sorbance between that for the antigen (GST-CpP23) well and that of the control antigen (GST) well. Sera Blood samples (n = 642) were collected from the caudal or jugular vein of dairy cows belonging to 42 small-holder farmers of the top three highest number of dairy cow population in Chiang Mai (150 sam- ples), Chiang Rai (392 samples) and Lumpang provinces (100 samples) (Fig. 1). Sera were sepa- rated after sedimentation of blood cells and were stored at –20 °C until use. RESULTS AND DISCUSSION The truncated CpP23 gene without sequences en- coding a hydrophobic signal peptide and a C-term- inus was inserted into the bacterial expression vec- tor pGEX-4T-3, and expressed as a GST fusion protein (GST-CpP23) in E. coli. The GST-CpP23 reacted strongly with sera from C. parvum-infected cattle but not with sera from uninfected cattle (data not shown). This result indicated that the GST- CpP23 can be adopted as a useful antigen for sero- diagnosis of C. parvum infection. The prevalence of C. parvum infection in cattle has been reported in many parts of the world, such as Canada (40.6 %) (Trotz Williams, Jarvie, Martin, Leslie & Peregrine 2005), USA (8.7 %) (Fay er, Trout & Graczyk 2000), Spain (8.4 %) (Cas tro-Hermida, Almeida, González-Warleta, Correia da Costa, Rumbo-Lorenzo & Mezo 2007), Australia (48 %) (Becher, Robertson, Fraser, Palmer & Thompson 2004), Japan (12 %) (Sakai, Tsushima, Nagasawa, Ducusin, Tanabe, Uzaka & Sarashina 2003) and Vietnam (33.5 %) (Nguyen, Nguyen, Le, Le Hua, Van Nguyen, Honma & Nakai 2007). In Thailand, most investigations have been carried out in hu- mans, but less is known of the infection in animals, particularly in dairy cows, which might be the carrier of the parasite. The ELISA with GST-CpP23 as antigen was used to investigate the seroprevalence of C. parvum in- fection in dairy cows in the northern part of Thailand. The overall seroprevalence of C. parvum infection was 4.4 % (28/642). This is lower than the preva- lence (9.4 %) in Nong Pho dairy areas (the central part of Thailand) as has previously been reported (Jittapalapong et al. 2006). The seropositive rates in three provinces were 3.3 % (5/150) in Chiang Mai, 5.1 % (20/392) in Chiang Rai and 3 % (3/100) in Lumpang (Table 1). Chiang Rai Province was the highest endemic area for C. parvum infection in this investigation. The numbers of dairy farm harbouring infected cows were from 16 to 42 (38 %) and the farm infection prevalence was 37.5 % (3/8), 37.9 % (11/29) and 40 % (2/5) in Chiang Mai, Chiang Rai and Lumpang respectively. A widespread infection rate in dairy cows due to C. parvum in the northern FIG. 1 Map of Thailand showing the location of the three prov- inces from which blood samples were collected: Chiang Mai Prov ince (CM), Chiang Rai Province (CR) and Lumpang Province (LP) 164 Cryptosporidium parvum infection of dairy cows in Thailand region of Thailand was therefore determined in this study. The seroprevalence of C. parvum infection rates varied in different age groups, ranging from 2.63 % to 14.29 % (Table 2). The age of the animal is one of the most important risk factors associated with cryptosporidiosis. However, the occurrence of C. par vum infection in the current study was found in all age groups but no statistically significant differ- ences between the age groups were determined. Nevertheless, it has been shown that asymptomatic adult domestic ruminants, such as dairy cows, sheep and goats may act as carriers and may be a source of infection for younger animals (Fayer et al. 2000; Bomfim, Huber, Gomes & Alves 2005). The current study demonstrated a low prevalence rate of C. parvum in dairy cows; however, asympto- matic cattle can serve as important natural reser- voirs for this parasite. These data also indicate a potential risk of C. parvum transmission to the hu- man population in Thailand and the need for more attention to be paid to its control in dairy cattle be- cause of its zoonotic nature. ACKNOWLEDGEMENTS We thank the provincial veterinary officers in the Department of Livestock Development in Chiang Rai, Chiang Mai and Lumpang provinces for their help in collecting the blood samples from the dairy farms. We also thank all the diary cow owners co- operated in this study. This project was financially supported by the Faculty of Veterinary Medicine, Kaset sart University Research Development Insti- tute (KURDI), the Japan International Cooperation Agency (JICA) and the Program of Founding Re- search Center for Emerging and Re-emerging Infectious Diseases, MEXT Japan. REFERENCES ABE, N., KIMATA, I. & ISEKI, M. 2002. Identification of geno- types of Cryptosporidium parvum isolated from a patient and dog in Japan. Journal of Veterinary Medical Science, 64:65– 168. 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TABLE 1 Seroprevalence of C. parvum infection in the dairy cows determined by ELISA Provinces C. parvum No. of samples No. of positive samples Seroprevalence (%) Chiang Rai Chiang Mai Lumpang 392 150 100 20 5 3 5.1 3.3 3.0 Total 642 28 4.4 TABLE 2 Seroprevalence of C. parvum infection in different age groups of the dairy cows or heifers Provinces Age (year) No. of animals No. of positive serum samples Seroprevalence (%) Chiang Mai < 1 > 1–5 > 5 11 96 43 0 5 0 0 5.21 0 Chiang Rai < 1 > 1–5 > 5 0 212 180 0 9 11 0 4.25 6.11 Lumpang < 1 > 1–5 > 5 7 76 17 1 2 0 14.29 2.63 0 165 T. INPANKAEW et al. CASTRO-HERMIDA, J.A., ALMEIDA, A., GONZÁLEZ-WAR- LETA, M., CORREIA DA COSTA, J.M., RUMBO-LORENZO, C. & MEZO, M. 2007. Occurrence of Cryptosporidium par- vum and Giardia duodenalis in healthy adult domestic rumi- nants. Parasitology Research, 101:1443–1448. CURRENT, W.L. & GARCIA, L.S. 1991. Cryptosporidiosis. Clin- ical Microbiology Reviews, 4:325–358. FAYER, R., TROUT, J.M. & GRACZYK, T.D. 2000. 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