Molecular Identification of Bovine Brucellosis Causing Organisms at Selected Private Farms in Pothohar Plateau, Pakistan
Molecular Identification of Bovine Brucellosis Causing Organisms at Selected Private Farms in Pothohar Plateau, Pakistan
Shahzad Ali1,*, Heinrich Neubauer2, Falk Melzer2, Iahtasham Khan1, Shamim Akhter3, Tariq Jamil2 and Sajid Umar3
1University of Veterinary and Animal Sciences (UVAS), Lahore, Pakistan
2Friedrich-Loeffler-Institute, Jena, Germany
3Pir Mehr Ali Shah-Arid Agriculture University, Rawalpindi, Pakistan
ABSTRACT
Brucellosis is a worldwide zoonotic infection in animals including Pakistan. A study was conducted to identify the potential cause of infection in three different cattle farms located at Potohar Plateau in Punjab, Pakistan. A total of 399 serum samples from indeginous and exotic cattle were tested for brucellosis by RBPT, SAT and multiplex real-time PCR for Brucella sp., Brucella abortus and Brucella melitensis. A total of 20 (5.01%) samples were found seropositive by RBPT and 19 (4.76%) by SAT, however real-time PCR showed 13 (3.25%) samples positive for both Brucella (sp.) and Brucella abortus. None of the seropositive samples were found positive for Brucella melitensis by real-time PCR. Exotic cattle tended to be more positive for the infection as compared to indigenous cattle. Routine screening and strict biosecurity measures are recommended for prevention of infection in animals. Humans must consume milk after pasteurization.
Article Information
Received 03 October 2016
Revised 11 November 2016
Accepted 28 January 2017
Available online 25 May 2017
Authors’ Contributions
SA, IK and SU collected the samples and analysed the data. SA, HN and FM wrote the article. TJ helped in preparation of the article.
Key words
Brucellosis, Brucella abortus, Real-time PCR, Cattle, Pothohar Plateau.
DOI: http://dx.doi.org/10.17582/journal.pjz/2017.49.3.sc2
* Corresponding author: shahzaduaar772@gmail.com
0030-9923/2017/0003-1111 $ 9.00/0
Copyright 2017 Zoological Society of Pakistan
Brucellosis is a worldwide zoonotic infection in a variety of animals e.g. cattle, buffaloes, sheep, goats and camels. It is primarily caused by Brucella abortus in bovines and Brucella melitensis in small ruminants whereas cross-species transmission of this infection is possible (Aparicio, 2013; Ali et al., 2015; Wareth et al., 2015). Characteristic signs include abortion in last trimester and retention of fetal membranes in female animals whilst orchitis and epididymitis in males, resulting overall in infertility (Corbel, 2006). Once infected, the bacteria are heavily shed in vaginal secretions and milk (Aparicio, 2013; Ebrahimi et al., 2014). In animals, this infection transmits directly via contact with infected animals or indirectly through ingestion of contaminated feed or water whereas in humans; it is through ingestion of contaminated raw milk or milk products (Mukhtar, 2010; Wareth et al., 2014; Ali et al., 2016). This infection is considered as endemic in Pakistan (Munir et al., 2011; Ali et al., 2014). The country bears a huge number of livestock i.e. 186.2 million among which ruminants (bovines, small ruminants and camels) make share of 180.5 million (96.9 %) (Anonymous, 2016). Current study was designed to investigate the infection status at three private farms located in Pothohar Plateau region by serological and molecular diagnostic techniques.
Materials and methods
Pothohar Plateau is located in north east of Pakistan consisting of four districts; Rawalpindi, Chakwal, Jhelum, Attock and Islamabad Capital Territory (ICT). It is surrounded by Jhelum River in the east, Indus River in the west, Margalla hills in north and the Salt range in south. This area falls under arid climate zone of Pakistan (Khan, 2004; Kazmi and Rasul, 2012). Livestock are mainly fed by grazing on range lands (Chaudary et al., 2007). Both indigenous and exotic cattle are prevalent with exotic animals raised primarily for milk production. However, intensive husbandry practices are only seen by exotic cattle.
A total of 399 blood samples (250 from indigenous and 149 from exotic cattle) were collected from three different livestock farms in the region. Blood samples (3 ml) were collected directly from jugular vein with a 5 ml syringe. Each blood sample was transferred into a non-EDTA coated vacutainer, placed at room temperature for 30 min, and centrifuged at 4,000 rpm for 15 min. Serum was discharged into a 1.5 ml Eppendorf tubes and stored at
Table I.- Primer/Probes Sequence for Brucella genus and species-specific real-time-PCR.
| Serial No. |
Sequence |
|
|
Brucella (genus) |
Forward primer | 5’-GCTCGGTTGCCAATATCAATGC-3’ |
| Reverse primer | 5’-GGGTAAAGCGTCGCCAGAAG-3’ | |
| Probe | FAM-AAATCTTCCACCTTGCCCTTGCCATCA-BHQ1’ | |
| Brucella abortus | Forward primer | 5’-GCGGCTTTTCTATCACGGTATTC-3’ |
| Reverse primer | 5’-CATGCGCTATGATCTGGTTACG-3’ | |
| Probe | FAM-CGCTCATGCTCGCCAGACTTCAATG-BHQ1 | |
| Brucella melitensis | Forward primer | 5’-AACAAGCGGCACCCCTAAAA-3’ |
| Reverse primer | 5’-CATGCGCTATGATCTGGTTACG-3’ | |
| Probe | FAM-CAGGAGTGTTTCGGCTCAGAATAATCCACA-BHQ1 | |
Table II.- Presence of B. abortus antibodies in different breeds of cattle using Rose Bengal Plate Test (RBPT).
| Cattle Breeds | Samples examined | Positive sample | Positive (%) |
| Achai | 13 | 0 | 0 |
| Cholistani | 24 | 1 | 4.17 |
| Dhani | 56 | 1 | 1.79 |
| Lohani | 98 | 6 | 6.12 |
|
Red Sindhi |
24 | 1 | 4.17 |
|
Sahiwal |
35 | 2 | 5.71 |
|
Holstein Frisian |
74 | 5 |
6.76 |
| Jersey | 75 | 4 |
5.33 |
-20 °C until further analysis.
Serum samples were screened initially by Rose Bengal Plate Test (RBPT) and then confirmed by Serum Agglutination Test (SAT) as described by Alton et al. (1988). Standard reagents were provided by Veterinary Research Institute (VRI), Lahore, Pakistan. A sample of 1:160 titers or higher was considered positive for SAT.
For molecular detection DNA was extracted from seropositive serum samples by using High Pure PCR Template preparation kit (Roche Diagnostic, Germany) as per manufacturer’s recommendations. DNA samples were stored at -20ºC till further analysis. Multiplex real-time PCR technique was used for molecular detection of the etiology as described by Probert et al. (2004).
Table I shows primers used for amplification of Brucella genus (bcsp31) and species (IS711 for B. abortus and B. melitensis). The cut-off cycle threshold (Ct) value for a positive sample was set as ≤ 40.
Results and discussion
A total of 20 (5.01%) serum samples were found seropositive by RBPT and 19 (4.76%) by SAT (Table II). Out of these sero-positive samples, 13 (overall 3.25%) were found positive only for both Brucella genus (BCSP31) and species Brucella abortus (IS711) by real time-PCR (Table III). None of these seropositive samples were found positive for Brucella melitensis. Only one sample, found positive by RBPT but negative by both SAT and real-time PCR, could be attributed to the low positive predictive value of RBPT (Gul and Khan, 2007).
Brucella abortus is a common etiology of brucellosis in bovines as well as in camels and small ruminants in the country (Ali et al., 2014, 2015; Fatima et al., 2016). Although open grazing, mixed farming and nomadic rearing pose brucellosis risk to animals, intensive farming also does not guarantee absolute protection (Gul and Khan, 2007; Abubakar et al., 2012; Ullah et al., 2015; Munir et al., 2011). Infected semen, breach in biosecurity and latent infection could be the main reasons. Recently, felines and canines have been reported to disseminate the infection at dairy farms (Wareth et al., 2016). Our study revealed the exotic animals tending to be more seropositive (6.04%) than indigenous animals (4.4%). Same results have been observed elsewhere in the country (Ali et al., 2013; Mangi et al., 2015; Kaleem et al., 2016) but one study has shown opposing results (Khan et al., 2016). These observations however, need to be studied further through intense inter-breed comparison of seropositive animals.
Table III.- Comparison of serological and molecular identification for detection of bovine brucellosis.
| Sample No | Cattle Breed |
Serological Tests |
|
qRT-PCR |
B. melitensis (IS711) | ||
|
RBPT |
SAT |
Brucella genus (BCSP31) |
B. abortus (IS711) |
||||
| 1 | Cholistani |
+ |
+ |
|
+ |
+ |
- |
| 2 | Dhani |
+ |
+ |
|
- |
- |
- |
| 3 | Lohani |
+ |
+ |
|
+ |
+ |
- |
| 4 | Lohani |
+ |
+ |
|
+ |
+ |
- |
| 5 | Lohani |
+ |
- |
|
- |
- |
- |
| 6 | Lohani |
+ |
+ |
|
+ |
+ |
- |
| 7 | Lohani |
+ |
+ |
|
- |
- |
- |
| 8 | Lohani |
+ |
+ |
|
- |
- |
- |
| 9 | Red Sindhi |
+ |
+ |
|
- |
- |
- |
| 10 | Sahiwal |
+ |
+ |
|
- |
- |
- |
| 11 | Sahiwal |
+ |
+ |
|
+ |
+ |
- |
| 12 | Holstein Frisian |
+ |
+ |
|
- |
- |
- |
| 13 | Holstein Frisian |
+ |
+ |
|
+ |
+ |
- |
| 14 | Holstein Frisian |
+ |
+ |
|
+ |
+ |
- |
| 15 | Holstein Frisian |
+ |
+ |
|
+ |
+ |
- |
| 16 | Holstein Frisian |
+ |
+ |
|
+ |
+ |
- |
| 17 | Jersey |
+ |
+ |
|
+ |
+ |
- |
| 18 | Jersey |
+ |
+ |
|
+ |
+ |
- |
| 19 | Jersey |
+ |
+ |
|
+ |
+ |
- |
| 20 | Jersey |
+ |
+ |
|
+ |
+ |
- |
Statement of conflict of interest
The authors declare no conflict of interest regarding this paper.
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