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Dive into the research topics where Arfan Ahmad is active.

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Featured researches published by Arfan Ahmad.


Virology Journal | 2013

Genetic diversity of Newcastle disease virus in Pakistan: a countrywide perspective

Muhammad Zubair Shabbir; Siamak Zohari; Tahir Yaqub; Jawad Nazir; Muhammad Abu Bakr Shabbir; Nadia Mukhtar; Muhammad Shafee; Muhammad Sajid; Muhammad Anees; Muhammad Abbas; Muhammad Tanveer Khan; Asad Ali; Aamir Ghafoor; Abdul Ahad; Aijaz Ali Channa; A. A. Anjum; Nazeer Hussain; Arfan Ahmad; Mohsan Ullah Goraya; Zahid Iqbal; Sohail Ahmad Khan; Hassan bin Aslam; Kiran Zehra; Muhammad Sohail; Waseem Yaqub; Nisar Ahmad; Mikael Berg; Muhammad Munir

BackgroundNewcastle disease (ND) is one of the most deadly diseases of poultry around the globe. The disease is endemic in Pakistan and recurrent outbreaks are being reported regularly in wild captive, rural and commercial poultry flocks. Though, efforts have been made to characterize the causative agent in some of parts of the country, the genetic nature of strains circulating throughout Pakistan is currently lacking.Material and methodsTo ascertain the genetics of NDV, 452 blood samples were collected from 113 flocks, originating from all the provinces of Pakistan, showing high mortality (30–80%). The samples represented domesticated poultry (broiler, layer and rural) as well as wild captive birds (pigeons, turkeys, pheasants and peacock). Samples were screened with real-time PCR for both matrix and fusion genes (1792 bp), positive samples were subjected to amplification of full fusion gene and subsequent sequencing and phylogenetic analysis.ResultsThe deduced amino acid sequence of the fusion protein cleavage site indicated the presence of motif (112RK/RQRR↓F117) typical for velogenic strains of NDV. Phylogenetic analysis of hypervariable region of the fusion gene indicated that all the isolates belong to lineage 5 of NDV except isolates collected from Khyber Pakhtunkhwa (KPK) province. A higher resolution of the phylogenetic analysis of lineage 5 showed the distribution of Pakistani NDV strains to 5b. However, the isolates from KPK belonged to lineage 4c; the first report of such lineage from this province.ConclusionsTaken together, data indicated the prevalence of multiple lineages of NDV in different poultry population including wild captive birds. Such understanding is crucial to underpin the nature of circulating strains of NDV, their potential for interspecies transmission and disease diagnosis and control strategies.


Journal of Virology | 2012

Complete Genome Sequencing of a Velogenic Viscerotropic Avian Paramyxovirus 1 Isolated from Pheasants (Pucrasia macrolopha) in Lahore, Pakistan

Muhammad Zubair Shabbir; Mohsan Ullah Goraya; Muhammad Abbas; Tahir Yaqub; Muhammad Abu Bakr Shabbir; Arfan Ahmad; Muhammad Anees; Muhammad Munir

ABSTRACT We report the complete genome sequence of avian paramyxovirus 1 (APMV-1) isolated from an acute and highly contagious outbreak in pheasants (Pucrasia macrolopha) in Lahore, Pakistan. Biological and serological characterization showed a velogenic strain of APMV-1, which was further confirmed by the sequence analysis of the cleavage site in the fusion protein. Complete genome sequencing and phylogenetic analysis indicated that this isolate belonged to genotype VII, specifically to subgenotype VIIa, and clustered closely with isolates characterized from Indonesia. Notably, the isolate showed significant differences from previously characterized APMV-1 from Pakistani commercial and rural chicken.


Journal of Parasitology | 2011

Seroprevalence of Neospora caninum and Brucella abortus in Dairy Cattle Herds with High Abortion Rates

Muhammad Zubair Shabbir; Muhammad Mudasser Nazir; Azhar Maqbool; Muhammad Lateef; Muhammad Abu Bakr Shabbir; Arfan Ahmad; Masood Rabbani; Tahir Yaqub; Muhammad Sohail; Muhammad Ijaz

abstract:  The protozoan Neospora caninum and the bacterium Brucella abortus are well-recognized causes of abortion in dairy cattle. Serum samples (n  =  240) from aborting (n  =  141) and at-risk (n  =  99) animals from 5 herds with high abortion rates in Punjab Province, Pakistan, were tested for antibodies to N. caninum using monoclonal antibody–based ELISA and for antibodies to B. abortus using the serum agglutination test. Antibodies to N. caninum and B. abortus were detected in 105 (43.8%) and 135 (56.3%) cattle, respectively. Prevalences of antibodies to N. caninum and B. abortus were higher in aborting cows (46.8% and 76.6%, P < 0.05) than in animals at risk (39.4% and 27.3%, P > 0.05). Sixty-six animals (27.5%) were seropositive to both N. caninum and B. abortus, and results showed no significant difference (P > 0.05) with respect to geographical district, breed, and age. This is the first report of N. caninum infection among dairy cattle herds in Pakistan.


Frontiers in Microbiology | 2015

Prevalence and distribution of soil-borne zoonotic pathogens in Lahore district of Pakistan

Muhammad Zubair Shabbir; Tariq Jamil; Asad Ali; Arfan Ahmad; Muhammad Naeem; Muhammad Hamid Chaudhary; Muhammad Bilal; Muhammad Ali; Khushi Muhammad; Tahir Yaqub; Asghari Bano; Ali I. Mirza; Muhammad Abu Bakr Shabbir; Walter R. McVey; Ketan Patel; Stephen Francesconi; Bhushan M. Jayarao; Masood Rabbani

A multidisciplinary, collaborative project was conducted to determine the prevalence and distribution of soil-borne zoonotic pathogens in Lahore district of Pakistan and ascertain its Public Health Significance. Using a grid-based sampling strategy, soil samples (n = 145) were collected from villages (n = 29, 5 samples/village) and examined for Bacillus anthracis, Burkholderia mallei/pseudomallei, Coxiella burnetii, Francisella tularensis, and Yersinia pestis using real time PCR assays. Chemical analysis of soil samples was also performed on these samples. The relationship between soil composition and absence or presence of the pathogen, and seven risk factors was evaluated. DNA of B. anthracis (CapB), B. mallei/pseudomallei (chromosomal gene), C. burnetii (IS1111, transposase gene), and F. tularensis (lipoprotein/outer membrane protein) was detected in 9.6, 1.4, 4.8, and 13.1% of soil samples, respectively. None of the samples were positive for protective antigen plasmid (PA) of B. anthracis and Y. pestis (plasminogen activating factor, pPla gene). The prevalence of B. anthracis (CapB) was found to be associated with organic matter, magnesium (Mg), copper (Cu), chromium (Cr), manganese (Mn), cobalt (Co), cadmium (Cd), sodium (Na), ferrous (Fe), calcium (Ca), and potassium (K). Phosphorous (P) was found to be associated with prevalence of F. tularensis while it were Mg, Co, Na, Fe, Ca, and K for C. burnetii. The odds of detecting DNA of F. tularensis were 2.7, 4.1, and 2.7 higher when soil sample sites were >1 km from animal markets, >500 m from vehicular traffic roads and animal density of < 1000 animals, respectively. While the odds of detecting DNA of C. burnetii was 32, 11.8, and 5.9 higher when soil sample sites were >500 m from vehicular traffic roads, presence of ground cover and animal density of < 1000 animals, respectively. In conclusion, the distribution pattern of the soil-borne pathogens in and around the areas of Lahore district puts both human and animal populations at a high risk of exposure. Further studies are needed to explore the genetic nature and molecular diversity of prevailing pathogens together with their seroconversion in animals and humans.


Acta Tropica | 2016

Evidence of Coxiella burnetii in Punjab province, Pakistan.

Muhammad Zubair Shabbir; Sidra Akram; Zia ul Hassan; Kashif Hanif; Masood Rabbani; Javed Muhammad; Muhammad Hamid Chaudhary; Tariq Abbas; Muhammad Taslim Ghori; Haroon Rashid; Tariq Jamil; Zia-ul Islam; Haisem Rasool; Asghari Bano; Arfan Ahmad; Muhammad Ali; Tahir Yaqub; Walt McVey; Bhushan M. Jayarao

Coxiella burnetii causes query (Q) fever, an important zoonotic disease with worldwide significance. The role of environment in the ecology of C. burnetti, and its influence on seroconversion in animals has not been elucidated in Pakistan. We carried out a cross-sectional study in Punjab province to (1) determine the prevalence and distribution of C. burnetii in soil using an ISIIII gene-based real time-polymerase chain reaction (RT-PCR) assay, (2) analyze association between the occurrence of C. burnetii in soil and its predictors i.e. soil characteristics (macro- and micro-nutrients) and several likely risk factors including the seroconversion in small ruminants at places where its genome had or had not been detected, and (3) predict homology and genetic diversity of the identified strains using sequences originated from different hosts worldwide. A total of 2425 soil samples from nine districts of Punjab province were processed. C. burnetii DNA was detected in 47 samples (1.94%, 95% CI: ±0.55) originating from 35 villages of studied districts (7.22%, 95% CI: ±2.30). The highest prevalence was found in Attock (7.11%, 95% CI: ±3.36), followed by Lahore (4.83%, 95% CI: ±3.49), Sahiwal (4.70%, 95% CI: ±2.6), Dera Ghazi Khan (2.33%, 95% CI: ±2.02), Faisalabad (1.35%, 95% CI: ±1.18) and Sheikhupura (0.68%, 95% CI: ±0.94). The odds of detecting bacterial DNA in soil was increased with a unit increase in organic matter [2.511 (95% CI: 1.453-4.340), p=0.001] and sodium [1.013 (95% CI: 1.005-1.022), p=0.001], whereas, calcium [0.984 (95% CI: 0.975-0.994), p=0.002] and potassium [0.994 (95% CI: 0.990-0.999), p=0.011] had protective effect where a unit increase in each analyte decreased odds for its occurrence by 1.0% approximately. Likewise, for categorical variables (risk factors), the odds of detecting C. burnetii were higher at locations >500m away from a main road [1.95 (95% CI: 1.06-3.78), p=0.04]. The enzyme-linked immunosorbent assay (ELISA) revealed an increased prevalence of antibodies in sheep (17.9%, 95% CI: ±5.54) compared with goats (16.4%, 95% CI: ±4.34). When determining the association between soil DNA and C. burnetii antibodies in small ruminants, the odds of detecting these antibodies were significant in sheep at the livestock barns [2.81 (95% CI: 1.20-7.37), p=0.02]. The IS1111 gene-based sequence analysis revealed a clustering of the DNA into two distinct groups with much genetic divergence (0.76-68.70%): the first group that contained sequences from Lahore district clustered with human and buffalo origin isolates, whereas the second group that contained the sequences from the remaining study districts clustered with goat-, rodent- and human-origin isolates. This study provides the first evidence of the presence of C. burnetii in the environment in Punjab province, Pakistan. Future studies are needed to ascertain the bacterias molecular epidemiology over a wide geographical area, type the isolates, and evaluates the potential risks to human populations, particularly farmers and veterinarians.


Journal of General Virology | 2016

Infectivity of wild bird-origin avian paramyxovirus serotype 1 and vaccine effectiveness in chickens

Muhammad Zubair Shabbir; Sameera Akhtar; Yi Tang; Tahir Yaqub; Arfan Ahmad; Ghulam Mustafa; Muhammad Azhar Alam; Diwakar Santhakumar; Venugopal Nair; Muhammad Munir

Newcastle disease virus, a prototype avian paramyxovirus serotype 1 (APMV-1), causes economically devastating disease in avian species around the world. Newcastle disease is enzootic in Pakistan and recurrent outbreaks are frequent in multiple avian species even after continuous and extensive use of vaccines. A number of APMV-1 and pigeon paramyxovirus serotype 1 (PPMV-1) strains have been isolated and genetically characterized in recent years. However, the impact of recently characterized wild bird-origin APMVs in domestic poultry, and the potency of routinely used vaccines against these novel and genetically diverse viruses remain unknown. Here, we applied next-generation sequencing for unbiased complete genome characterization of APMV-1 and PPMV-1 strains isolated from clinically diseased peacocks (Pavocristatus) and pigeons (Columbalivia), respectively. Global phylodynamics and evolutionary analysis demonstrates Pigeon/MZS-UVAS-Pak/2014 is clustered into lineage 4 (or genotype VI) and Peacock/MZS-UVAS-Pak/2014 into lineage 5 (or genotype VII). The genomes of both isolates encoded for polybasic residues (112RRQKR↓F117) at the fusion protein cleavage motif along with a number of important substitutions in the surface glycoproteins compared with the vaccine strains. Clinicopathological and immunological investigations in domesticated chickens indicate that these isolates can potentially transmit between tested avian species, can cause systemic infections, and can induce antibodies that are unable to prevent virus shedding. Collectively, the data from these genomic and biological assessments highlight the potential of wild birds in transmitting APMVs to domesticated chickens. The study also demonstrates that the current vaccine regimens are incapable of providing complete protection against wild bird-origin APMVs and PPMVs.


international bhurban conference on applied sciences and technology | 2017

Association of soil chemistry and other factors with spatially distributed Burkholderia mallei DNA in Punjab province, Pakistan

Muhammad Ali; Khushi Muhammad; A. A. Anjum; Mansur-ud-Din Ahmad; Masood Rabbani; Muhammad Zubair Shabbir; Arfan Ahmad; Muhammad Nawaz; Muhammad Tasleem Ghori; Javed Muhammad; Haroon Rashid Chaudhry; Tariq Jamil; Muhammad Haisem; Tasmia Awan; Rais Ahmad; Bhushan M. Jayarao

Association of soil chemistry and other risk factors with soil borne Burkholderia mallei (B. mallei) DNA in eight districts (Sheikhupura, Gujranwala, Faisalabad, Sargodha, Chakwal, Attock, Sahiwal, Dera Ghazi Khan) of Punjab province, Pakistan, was studied. A total of 22 soil samples (n=11, each from soil positive and negative for B. mallei DNA) were processed for chemical analysis from B. mallei positive districts (Sheikhupura and Chakwal). The relationship between soil composition, absence or presence of the pathogen was ascertained. In soil samples of Chakwal district, DNA of B. mallei was found to be highly associated with 0.80 to 39.20% range of moisture contents (p=0.008) and 1.74 to 21.75 mg/Kg of P (p=0.050). The association in Sheikhupura district was with sodium (1.90 to 133.59 mg/Kg; p=0.018) and moisture (0.80 to 39.20%; p=0.026). The odds of detecting DNA of B. mallei was 1.4, 6.8, 5.0, 2.8 and 10.6 higher when soil sample sites were < 500 meters from vehicular traffic roads, < 01 km from animal markets, < 100 meters from canal, < 1000 animals and < 300 houses/village, respectively. While the odds of detecting DNA of B. mallei were 0.1, 0.3, 0.4, 0.2 and 0.5 when soil sample sites were > 500 meters from vehicular traffic roads, > 01 km from animal markets, > 100 meters from canal, > 1000 animals and > 300 houses/village. Soilborne B. mallei DNA is more likely to be detected in areas closer to roads having vehicular traffic along with interstate routes and soil containing low levels of moisture.


Pakistan Veterinary Journal | 2013

Zoonosis update on H9N2 avian influenza virus.

Abdul Ahad; Masood Rabbani; Altaf Mahmood; Z. H. Kuthu; Arfan Ahmad; Mustafizur Rahman


Pakistan Veterinary Journal | 2013

Serological evidence of selected abortifacients in a dairy herd with history of abortion.

Muhammad Zubair Shabbir; R. K. Khalid; D. M. Freitas; Maryam Javed; Masood Rabbani; Tahir Yaqub; Arfan Ahmad; Muhammad Asim Shabbir; Muhammad Abbas


International Journal of Agriculture and Biology | 2008

Immunomodulatory effect of Polyimmune (Astragalus membranaceus) extract on humoral response of layer birds vaccinated against Newcastle disease virus.

Muhammad Zubair Shabbir; Aamir Ghafoor; Arfan Ahmad; A. A. Anjum; Tahir Yaqub

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Masood Rabbani

University of Veterinary and Animal Sciences

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Muhammad Zubair Shabbir

University of Veterinary and Animal Sciences

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Tahir Yaqub

University of Veterinary and Animal Sciences

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Khushi Muhammad

University of Veterinary and Animal Sciences

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A. A. Anjum

University of Veterinary and Animal Sciences

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Muhammad Ali

University of Veterinary and Animal Sciences

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Javed Muhammad

University of Veterinary and Animal Sciences

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Muhammad Abu Bakr Shabbir

University of Veterinary and Animal Sciences

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Tariq Jamil

University of Veterinary and Animal Sciences

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Bhushan M. Jayarao

Pennsylvania State University

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