Seroprevalence of Brucellosis in Holstein-Friesian and Indigenous Cattle Breeds of Sindh Province , Pakistan

| Brucellosis is considered to be one of the most widespread zoonosis in the world. A comparative study on the seroprevalence of brucellosis in indigenous cattle breeds and exotic cattle (Holstein-Friesian) was carried out in district Hyderabad, Sindh, Pakistan. A total of 500 serum samples, 100 each from Red Sindhi, Thari, Kankrej, Bhagnari and Holstein-Friesian breeds were collected from both male and female animals and examined by Rose Bengal plate test (RBPT), serum agglutination test (SAT) and Competitive Enzyme Linked Immunosorbent Assay (c-ELISA). The overall prevalence of brucellosis in cattle was determined as 25, 23.2 and 11.8% by RBPT, SAT and c-ELISA respectively. However, highest prevalence of brucellosis was recorded in Holstein-Friesian (RBPT: 35%; SAT: 33%; c-ELISA: 17%), followed by Red Sindhi (RBPT: 28%; SAT: 26%; c-ELISA: 15%), Thari (RBPT: 24%; SAT: 23%; c-ELISA: 9%), Kankrej (RBPT: 20%; SAT: 18%; c-ELISA: 10%) and Bhagnari (RBPT: 18%; SAT: 16%; c-ELISA: 8%). The sex-wise comparison of seropositive animals indicated that the prevalence of brucellosis was 26.88% in females and 8% in males by both, RBPT and SAT. Furthermore somewhat lower prevalence (12.22%) of brucellosis was demonstrated in female cattle by c-ELISA. The effect of age on the seroprevalence of brucellosis in cattle of Sindh province was also studied. Of the 250 sera examined from cattle ≤ 4 years of age, 51(20.4%), 49(19.6%) and 26 (10.4%) were found positive by RBPT, SAT and c-ELISA respectively. While, of the 250 sera of ˃ 4 years of age 74 (29.6%), 66 (26.4%) and 33 (13.2%) were found positive by RBPT, SAT and c-ELISA, respectively. It was concluded from the present study that exotic cattle (Holstein-Friesian) have higher seroprevalence of brucellosis compared to local cattle breeds amongst which highest prevalence was recorded in Red Sindhi and lowest in Bhagnari breed. Further, among the sero-diagnostic techniques applied during present investigation, the c-ELISA was found as superior technique to determine brucellosis in cattle.

ease is known to cause morbidity and considerable losses of productivity (Pappas, 2006).The disease is important from economic point of view, because it is one of the most devastating trans-boundary animal disease and also a major barrier for trade (Gul and Khan, 2007).
Brucellosis is a bacterial disease that caused by the organisms of genus Brucella.These are non-motile, anaerobic, intracellular pathogens ( Jarvis et al., 2002) that are usually found in the reticulo-endothelial and reproductive systems.Brucella replicate and persist in cells often resulting in infection or carrier state and also impair innate and adaptive immunity (Fichi, 2003).At least six species of the genus Brucella are recognized to be pathogenic for livestock worldwide.Among these, Brucella abortus is known as causative agent of bovine brucellosis (Corbel, 1998).
For the diagnosis of brucellosis in farm animals, bacteriological, serological and molecular methods are used.However, among these bacteriological and molecular tools like polymerase chain reaction are not widely used due to time consuming and economic issues, respectively.However, serological tests like milk ring test, Rose Bengal plate test etc., are most economical approaches, hence used widely for screening and monitoring of brucellosis in dairy cattle (Ali et al., 2013).
Cattle have been found more resistant to bovine brucellosis than buffaloes (Kamboh et al., 2007).Moreover, inter-breed differences in susceptibility to brucellosis are also reported for both cattle and buffaloes (Ali et al., 2013).However, no information is available about the susceptibility level of indigenous cattle breeds of Sindh province of Pakistan for brucellosis.Therefore, the present study was designed to investigate the seroprevalence of brucellosis in four indigenous and one exotic cattle breeds of Sindh province using three serological techniques.

ColleCtion of blood saMPles
A total of 500 blood samples were collected from different cattle breeds, i.e., 100 each from Red Sindhi, Thari, Kankrej, Bhagnari and Holstein-Friesian.These were collected from peri-urban private farms and taken from both males (n=10) and females (n=90) from district Hyderabad, Sindh, Pakistan.The blood samples from the animals were obtained through jugular vein by using disposable sterilized plastic syringes.The blood samples were transported in cool chain to the laboratory where the sera were separated by centrifugation at 200 g for 15 minutes.The sera were stored at -20˚C until analysed for Brucella antibodies.

rose bengal Plate test (rbPt)
For Rose Bengal plate test (RBPT), stained Brucella antigens (strain-99) were purchased from Veterinary Research Institute (VRI), Lahore.The antigens were used according to manufacturer's instructions and test procedure was adopted as described by Morgan et al. (1978).In brief, a drop of serum sample and a drop of Rose Bengal antigen were added in a well of the porcelain plate.The contents of both drops were mixed thoroughly and the reaction was observed after four minutes.Complete agglutination was recorded as positive and matched with positive and negative controls for confirmation.

seruM agglutination test (sat)
Serum agglutination test (SAT) was performed using the procedures described by Stemshorm et al. (1985).In brief, 0.8 ml of phosphate buffer saline (PBS) containing 0.5% phenol was added in clear glass tubes of approximately 2 ml volume.A 0.2 ml of test serum was added to first tube, mixed and then 0.5 ml was transferred to the next tube.After mixing well, 0.5ml was transferred to the third and so on up to the last fifth tube.An equal volume (0.5 ml) of standardized B. abortus antigen with phenol saline dilution (1:20) was added and the tubes were incubated overnight at 37˚C.The results of agglutination in SAT test tubes were determined by reading the degree of sedimentation in the tubes.A titre of 1:40 or more was considered as positive, titre of 1:20 was considered a doubtful and the titre of 1:10 was treated as negative.

Brucella C-elisa antibody test
In this assay, an ELISA kit (SVANOVIR Brucella-Ab I-ELISA, Sweden) was used according to manufacturer instructions.Briefly, a 4 µl of positive and negative control serum were added to selected wells coated with Brucella antigen.An equal volume (4 µl) of serum sample was added to the selected well coated with Brucella antigen.The plate was thoroughly shacked, sealed and incubated at 37˚C for one hour.Then rinsed 3 times with PBS-Tween buffer.A 100 µl of Horse reddish peroxidase (HRP) conjugate was added to each well and incubated at 37˚C for 1 hour.The plate was again rinsed thrice, and 100 µl substrate solution (Tetra methyl benzidine) was added to all wells.The plate was incubated for 10 minutes, at 25˚C.Finally, reaction was stopped by adding 50 µl of stop solution to each well and mixing thoroughly.The optical density (OD) of the control and test sample wells was measured at 450 nm using a micro plate photometer (Thermo Electron, Finland).The OD was measured within 15 minutes after adding the stop solution to prevent the fluctuation in the OD values.All results were calculated in terms of PP (Percentage Positivity) value and interpreted accordingly.The sera sample showing PP value lesser than 15, was considered negative and those showing PP value equal or greater than 15, was known as positive.All the samples were run in duplicates.

data analysis
All results are expressed in percentages that were calculated

seroPreValenCe of bruCellosis within gender of Various Cattle breeds
A total of 50 serum samples from male and 450 from female animals were analysed by RBPT, SAT and c-ELISA to record the gender-wise seroprevalence of brucellosis in cattle and data were presented in  2009) conducted a study on Holstein cattle of a small scale dairy production system for Brucella abortus antibodies in Cameroon by ELISA and found a general seroprevalence of 8.4% in Holstein cattle.These differences in seroprevalence of bovine brucellosis might be due to geographical variations, or difference in the animal species (cattle or buffalo) used in study (Ansari et al., 2014;Sachan et al., 2013).Likewise, in a recent study by our laboratory, regarding prevalence of bovine brucellosis, it was found that Brucella abortus specific antibodies have higher ratio in buffalo (47/100) than cattle (31/100) (Soomro et al., 2014).We have also documented the geographical variations in our previous studies (Kamboh et al., 2007;Durrani et al., 2015) for prevalence of bovine brucellosis that might be of nutritional or managemental origin.
Our study have investigated first time, the inter-breed differences for seroprevalence of brucellosis in different local and exotic breeds of cattle.We found highest prevalence of B. abortus antibodies in exotic breed i.e., Holstein-Friesian cattle followed by Red Sindhi, Thari, Kankrej and Bhagnari.These results indicated that our local cattle breeds have resistance for Brucella infection compared to exotic breed.However, this finding needs further investigation especially using the advanced molecular approaches.In similar study in Bangladesh, seroprevalence of brucellosis was reported to be 6.28% in cross breed cattle comparing with 0.85% in local breeds (Sikder et al., 2012).On the contrary, Omer et al. (2000)  An investigation on the seroprevalence of brucellosis in different sexes of all cattle breeds was carried out.The prevalence of brucellosis was detected 26.88% in females by RBPT and 24.88% by SAT.Furthermore, somewhat lower prevalence of brucellosis was demonstrated in female (12.22%) cattle by c-ELISA.On the other hand, interestingly, in males all three techniques indicated the similar level of disease prevalence, this might be due to lesser number of samples used in this study as compared to females.All techniques applied during investigation detected 2-3 times higher prevalence of brucellosis in females as compared to males.It is evident from the study that females are at higher risk of brucellosis than the males.This might be due to males getting infected from Brucella species that could infect a large number of females.Furthermore, this might be due to opening of cervix during estrus for more than a week gets infected from Brucella bacterial species.A higher seroprevalence of bovine brucellosis in females has also been reported by other studies including Malik et al. (2013) who reported an overall seroprevalence of brucellosis in bovine population as 21.36%, with significant (p<0.01)differences in respect to sex (male, 1.81% and female 28.69%).Similarly, Adamu et al. (2014) also found a higher seroprevalence of bovine brucellosis in females (18.0%) than males (5.0%).
We have also evaluated the effect of age on the seroprevalence of brucellosis in cattle of Sindh province, and found high prevalence in older (≥4 year) cattle regardless of technique.The reason of higher prevalence of brucellosis in older animals might be due to lesser immunity because the cattle are in lactating stage.Higher seroprevalence of brucellosis in older age groups of cattle has been reported by several studies.Junaidu et al. (2006) reported a higher (12.4%) sero-prevalence of brucellosis in cattle with the age ranging from 5.5 -10 years.Abou-Eisha, (2000) also recorded a higher prevalence (3.98%) of brucellosis in animals over 5 years of age.Similarly, Adamu et al. (2014) determined a higher prevalence of 9.5% in animals of Rose Bengal plate test; SAT: serum agglutination test; c-ELISA: Competitive Enzyme Linked Immunosorbent Assay; * Number of samples analyzed in each test = 90; ** Number of samples analysed in each test = 10

Figure 1 :
Figure 1: Seroprevalence of brucellosis in various cattle breeds determined by different techniques n= 100 for RBT, SAT and c-ELISA; n=500 for total; RBPT= Rose Bengal plate test; SAT= Serum agglutination test; c-ELISA= Competitive Enzyme Linked Immunosorbent Assay by dividing the number of positive samples with total number of samples x100, using Microsoft Office Excel 2010.

Table 1 :
The seroprevalence of brucellosis within gender of various cattle breeds determined by various techniques

seroPreValenCe of bruCellosis within different age grouPs of Cattle breeds
Table1.The prevalence of brucellosis was detected 26.88% by RBPT, 24.88% by SAT and 12.22% by c-ELISA in female animals.However, similar level of prevalence was observed in males i.e., 8.00% by all three techniques.cattle≤4years of age (Table2).Among 250 examined sera samples from cattle ≤4 years of age, 51 (20.4%), 49 (19.6%) and 26 (10.4%) were found positive by RBPT, SAT and c-ELISA respectively.On the other hand, when 250 sera were collected and tested from cattle >4 years of age, 74 Journal of Animal Health and Production October 2015 | Volume 3 | Issue 4 | Page 85 (OIE, 2008)gher prevalence of brucellosis among mixed breeds of cattle compared to indigenous breeds in Asmara region of Eritrea.During present investigation, we have also compared the diagnostic techniques i.e., RBPT, SAT and c-ELISA for their sensitivity.The results indicated that the highest prevalence of brucellosis was detected by RBPT and SAT in all five breeds of cattle.However, RBPT and SAT have been reported to produce false positive results due to cross reaction with antibodies of other bacterial species whereas in c-ELISA there is much lesser probability of both false positive or negative results(OIE, 2008).