Bovine herpesvirus-1 (BHV-1) a re-emerging concern in livestock: a revisit to its biology, epidemiology, diagnosis, and prophylaxis

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1 Veterinary Quarterly ISSN: (Print) (Online) Journal homepage: Bovine herpesvirus-1 (BHV-1) a re-emerging concern in livestock: a revisit to its biology, epidemiology, diagnosis, and prophylaxis Suman Biswas, Samiran Bandyopadhyay, Umesh Dimri & Pabitra H. Patra To cite this article: Suman Biswas, Samiran Bandyopadhyay, Umesh Dimri & Pabitra H. Patra (2013) Bovine herpesvirus-1 (BHV-1) a re-emerging concern in livestock: a revisit to its biology, epidemiology, diagnosis, and prophylaxis, Veterinary Quarterly, 33:2, 68-81, DOI: / To link to this article: Copyright Taylor and Francis Group, LLC Accepted author version posted online: 13 May Published online: 13 May Submit your article to this journal Article views: 2055 View related articles Citing articles: 16 View citing articles Full Terms & Conditions of access and use can be found at Download by: [ ] Date: 02 December 2017, At: 06:02

2 Veterinary Quarterly, 2013 Vol. 33, No. 2, 68 81, REVIEW ARTICLE Bovine herpesvirus-1 (BHV-1) a re-emerging concern in livestock: a revisit to its biology, epidemiology, diagnosis, and prophylaxis Suman Biswas a, Samiran Bandyopadhyay b, Umesh Dimri a and Pabitra H. Patra c a Division of Medicine, Indian Veterinary Research Institute, Izatnagar, Bareilly, India; b Eastern Regional Station, Indian Veterinary Research Institute, Kolkata, India; c Department of Pharmacology & Toxicology, C.V.Sc. & AH, Tripura, India (Received 30 January 2013; final version received 22 April 2013) Bovine herpesvirus-1 (BHV-1) is known to cause several diseases worldwide. It is a double-stranded DNA virus consisting of 33 structural proteins out of which 13 are associated with the envelope. Based on genomic analysis and viral peptide patterns, BHV-1 virus can be divided into several subtypes like BHV-1.1, BHV-1.2, and BHV-1.3. However, all subtypes are antigenically similar. The symptoms of the related diseases are mainly non-life-threatening but have a rather wide host range that limits animal trade. The different modes of transmission as unique feature of this virus and the tendency to cause infection in the early age with latency development in trigeminal and sacral ganglion cause huge economic losses around the world. The virus also affects endangered bovine species like mithun (Bos frontalis) and yak (Poephagus grunniens). The disease can be diagnosed by using conventional procedures (like cell culture, immune-histopathology, and enzymelinked immunosorbent assay (ELISA)) as well as highly sensitive modern techniques (like nested PCR and southern hybridization) with the virus neutralization test regarded as gold standard. With the currently available diagnostic tests it is not possible to identify animals which have a latent BHV-1 infection. Different types of modern and conventional vaccines are available for immunoprophylaxis. Inactivated vaccines are not as efficacious as modified live virus (MLV) vaccines. Marker vaccines allow the distinction between vaccinated and naturally infected animals. In this review the present status of BHV-1 around the world will be addressed besides the current knowledge with regard to its biology, epidemiology, diagnosis, and prophylaxis. Keywords: bovine; cattle; mithun; yak; BHV-1; vaccination; review 1. Introduction Bovine herpesvirus-1 (BHV-1) belongs to the genus Varicellovirus in the subfamily Alphaherpesvirinae under the family Herpesviridae. The virus is responsible for severe economic damage to the cattle industry throughout the world. The clinical spectrum of the disease is complex and the severity of the infection and pathogenesis depends upon its virulence. Development of latency is a unique feature of the virus. In most cases, the carrier animals go unnoticed and remain silent shedders of the pathogen and a potent source of infection for other animals on the farm. Thus, the pathogen continues to exist in the environment unnoticed and inflicting major damage to the livestock. Usually, the infection is not life threatening but secondary bacterial infection may complicate the scenario. Even though mortality is low, the disease with its severe impact on growth, milk production, and international livestock trade may jeopardize the agro-economy of a country. segment of approximately kbp with inverted repeat regions of approximately 24 kbp (Mayfield et al. 1983; Wyler et al. 1989; Schwyzer & Ackermann 1996). These UL, US, and inverted repeat regions are responsible for two isomeric forms of the viral genome (Mayfield et al. 1983). Based on the genomic analysis and viral peptide patterns, BHV-1 virus can be divided into several subtypes like BHV-1.1, BHV-1.2, and BHV-1.3. BHV- 1.1 mostly is related to the respiratory syndrome, BHV- 1.2 is related to genital infections, and BHV-1.3/BHV-5 is associated with neurological disorders of the cattle (Muylkens et al. 2007). However, all subtypes are antigenically similar. Antigenically BHV-1 is closely related to cervine herpesvirus-1 (CvHV-1), buffalo herpesvirus-1, and elk herpesvirus (Keuser et al. 2004)(see Table 1 and Figure 1). It is an enveloped virus and susceptible to disinfectants which destroy its lipid envelope. The virus can be isolated with the help of bovine cell cultures as well as cell lines of other species. 2. The virus 2.1. Subtypes BHV-1 is a double-stranded DNA virus having kbp size (Mayfield et al. 1983; Wyler et al. 1989), and codes for 70 proteins. The genomic sequence of the virus can be divided into a unique long (UL) segment of approximately kbp and a unique short (US) 2.2. Viral genome and proteins Herpesviruses are large, enveloped, double-stranded DNA viruses (Harrison 2001). Typical herpesvirus virions consist of a core containing linear double-stranded DNA and an icosadeltahedral capsid of about 100 nm diameter containing 162 capsomeres. The viral DNA genome is wrapped around a fibrous spool-like core, which has the *Corresponding author. udimrimesh@rediffmail.com Ó 2013 Taylor & Francis

3 Veterinary Quarterly 69 Table 1. Different prototypes of Herpesviridae, host range, and their associated infection in animals. Virus Host Species (heterologous) Disease Alphaherpesviridae subfamily Bovine herpesvirus-1 Cattle (goat, sheep, red deer, Infectious bovine rhinotracheitis rein deer) Bovine herpesvirus-2 Cattle and African ruminants Pseudo-lumpy skin disease, Allerton disease, bovine herpes mammilitis Bovine herpesvirus-5 Cattle (goat, sheep) Bovine encephalitis Suid herpesvirus-1 Swine (wild boar, Fatal encephalitis ruminants, carnivores) Cervid herpesvirus-1 Red deer Ocular disease Cervid herpesvirus-2 Rein deer (cattle) Subclinical genital infection Caprine herpesvirus-1 Goat (cattle, sheep) Genital disease, fatal neonatal disease Bubaline herpesvirus-1 Buffalo Subclinical genital infection Elk herpesvirus-1 Elk (cattle) Subclinical genital infection Ovine herpesvirus-1 Sheep Isolated in ovine pulmonary adenomatosis Gammaherpesviridae subfamily Bovine herpesvirus-4 Cattle, buffalo (ruminants, outmonkey, cat) shape of a torus. Surrounding the capsid is a layer of globular material, known as the tegument, which is enclosed by a typical lipoprotein envelope with numerous small glycoprotein spikes (Roizman et al. 2007; MacLachlan & Dubovi 2010). The US sequence is flanked by inverted internal repeat (IR) and terminal repeat (TR) sequences. In BHV-1 genome, a total of 73 open reading frames (ORF) coding for proteins have been identified. BHV-1 genome codes for 33 structural proteins, 13 of which are probably associated with the envelope (Liang et al. 1996) and 10 of these have the potential to encode glycoproteins (Schwyzer & Ackermann 1996). Among the 10 glycoproteins, six are in the UL segment, namely gk (UL53), gc (UL44), gb (UL27), gh (UL22), gm (UL10), and gl (UL1), whereas the four remaining ones are in the US segment, namely gg (US4), gd (US6), gi (US7), and ge (US8) (Muylkens et al. 2007). The other major proteins of BHV-1 are vhs (virion host shut down), VP8, VP16, BICP0, and BICP4 protein. The functions of some of the major proteins are given in Table Physiochemical properties of the virus BHV-1 is resistant to environmental influences. Inactivation of the virus in the environment depends on factors such as temperature, ph, light, and humidity. At 4 C, the virus is stable for 1 month. BHV-1 is inactivated at 56 C within 21 minutes, at 37 C within 10 days and at 22 C within 50 days (Gibbs & Rweyemamu 1977). The virus may survive for more than 30 days in feed. As the virus is enveloped, it is sensitive to organic solvents such as chloroform, ether, and acetone. The virus is sensitive to many disinfectants and is readily inactivated by 0.5% NaOH, 0.01% HgCl 2, 1% chlorinated lime, 1% phenolic derivatives, 1% quaternary ammonium bases, and 10% Lugol s iodine. Formalin (5%) inactivates BHV-1 within 1 minute (Straub 1990; Nandi et al. 2009). Subclinical infection, Vulvovaginitis, Bovine clinical and subclinical mastitis Ovine herpesvirus-2 Sheep (cattle, pig) Malignant catarrhal fever (in Europe) Alcelaphine herpesvirus-1 Wildebeest (cattle) Malignant catarrhal fever (in Africa) Alcelaphine herpesvirus-2 Hartebeest (cattle) Atypical malignant catarrhal fever 2.4. Host range BHV-1 primarily affects cattle. Other Artiodactyla (e.g. goats, sheep, water buffaloes, and camelids) may be infected with BHV-1. BHV-1 has been shown to infect and cause disease in sheep and goats also (Whetstone & Everman 1988). Antibodies to BHV-1 have been detected in captive Asian elephants (Elephas maximus) without any apparent clinical symptoms (Metzler et al. 1990; Bhat et al. 1997). BHV-1 has also been isolated from apparently healthy pronghorn antelope, wildebeest, mink, and ferrets (Porter et al. 1975) as well as from the soft-shelled tick Ornithodoros coriaceus (Taylor et al. 1982). Face flies (Musca autumnalis) can carry BHV-1, but they do not transmit the virus to the cattle (Johnson et al. 1991). BHV- 1 does not infect mice, rats, guinea pigs, or chick embryos (Gibbs & Rweyemamu 1977), although immunocompromised mice that lack interferon receptors can be infected if the virus is injected into the peritoneal cavity (Abril et al. 2004). Rabbits can be experimentally infected with BHV-1 if the virus is injected into the conjunctival sac of their eyes (Rock & Reed 1982; Rock et al. 1987, 1992), or through holes drilled into the sinuses (Brown & Field 1990a, 1990b). In vitro studies in cell culture showed that BHV-1 can bind weakly to human vascular endothelial cell (HveC) (nectin-1) or to the human poliovirus receptor (Geraghty et al. 1998; Connolly et al. 2001) without detectable viral replication. There are no reports of human infection with BHV Virus transmission BHV-1 is shed in nasal discharge for days during acute respiratory infection (Gibbs & Rweyemamu 1977) and transmission occurs by contact with mucosal droplets from infected cattle (Kahrs 2001). The virus is also shed following reactivation from latency. BHV-1 can also be

4 70 S. Biswas et al. Table 2. Function of some of the major proteins of the bovine herpesvirus-1. Sl. No. Protein name Function 1 gb (glycoprotein gb) Attachment, entry, direct cell-to-cell spread and fusion 2 gc (glycoprotein gc) Attachment 3 gd (glycoprotein gd) Entry, cell-to-cell spread 4 gi (glycoprotein gb) Cell-to-cell spread 5 gh (glycoprotein gh) Cell-to-cell spread 6 Vhs (virion host shut off) Rapid shut off of host cell protein synthesis 7 VP16 (a TIF - transinducing factor of alpha genes) Transactivator of BHV-1 immediate early (IE) genes 8 BICP0 Activator of viral promoters 9 VP8 Protein kinase; enhances a TIF function 10 BICP4 Transactivator of some gene promoters Figure 1. Phylogenetic relationships between animal alphaherpesviruses (gb: Glycoprotein B, ge: glycoprotein E). Available sequences from NCBI database were aligned using the Mega 4.1 program. The phylogenetic tree was obtained by unweighted pair group method with arithmetic mean (UPGMA) analysis. The phylogenetic distance was estimated by Kimura s two-parameter method using 1000 bootstrap replicates. Virus classification: Family: Herpesviridae; Subfamily: Alphaherpesvirinae; Species: Bovine herpesvirus 1 Genus: Varicellovirus. Dendrogram showing genetic diversity among the animal herpesviruses, isolated from different animals, based on the sequences of glycoprotein B. Dendrogram showing genetic diversity among the animal herpesviruses isolated from different animals based on the sequences of glycoprotein E.

5 Veterinary Quarterly 71 transmitted to susceptible animals through contaminated materials including semen (Mars et al. 2000). Airborne transmission of BHV-1.1 can occur under experimental conditions at distances of 3.85 meters (Wentink et al. 1993), and is dependent on environmental temperature and relative humidity (Elazhary & Derbyshire 1979; Mars et al. 1999). Till date, no vectors have been described for BHV Virus entry into host cells Herpesviruses enter cells by fusing with the cell plasma membrane in a complex process of attachment and penetration. Virus entry requires the presence of complementary binding partners on the virus and on the host cell. Studies show that the BHV-1 glycoproteins gb, gc, gd, ge, gh, gk, and gl are required for the virus entry (Li et al. 1995; Dasika & Letchworth 1999; Hanon et al. 1999; Schroder & Keil 1999). BHV-1.1 and BHV-1.2 subtypes differ in gc epitopes, which may alter viral attachment and virulence (Rijsewijk et al. 1999). Although the host cell proteins required for BHV-1 entry are not fully understood, the virus initially binds to cell surface heparan sulphate (Hanon et al. 1998; Tyler & Nathanson 2001) via BHV-1 gb and gc (Li et al. 1996). After this initial binding, BHV-1 gb and gd bind further quite strongly to cell surface receptors (Li et al. 1995). The nature and properties of these receptors are yet to be determined. Studies have shown that BHV-1 gd can weakly bind HveC or the human poliovirus receptor expressed in human or hamster cell lines (Geraghty et al. 1998; Connolly et al. 2001). This weak binding indicates that viral entry in a natural host may be mediated by receptors other than bovine HveC or poliovirus receptor homologues (Geraghty et al. 1998; Connolly et al. 2001) Virus replication and release After entry into the host cell, BHV-1 is transported along microtubules to the nucleus for replication using host cell proteins. The virus becomes enveloped as it buds through the nuclear envelope and is then transported within intracellular vesicles to the cytoplasmic membrane and released from the cell (Hunter 2001; Knipe et al. 2001). BHV-1 replication starts within 2 hours of infection in the cattle (Meurens et al. 2004b) with concomitant cell surface antigen expression within 3 4 hours after infection. Following assembling, the virus is released and it starts to infect other cells within 8 hours (Babiuk et al. 1996) Latency development Establishment of latency is a unique feature of this virus. BHV-1 virus can become latent following a primary infection with a field isolate or vaccination with an attenuated strain (Nandi et al. 2009). Latency is believed to develop in almost all animals that are infected with high or low doses of attenuated or virulent BHV-1 (Pastoret et al. 1982). Attenuated vaccine strains can remain in a latent state in the body and vaccination does not provide protection against establishment of a latent infection with a wild strain (Jones et al. 2000). Inoculation with live vaccine strains of BVH-1 can also lead to latent infection (Kit et al. 1985; SCAHW 2000). Vaccination in latently infected animals does not prevent re-excretion of a wild strain either. Young calves can have latent infections and have antibody responses due to infection in the presence of maternal antibodies (SCAHW 2000). Colostral anti- BHV-1 antibodies do not prevent initial virus replication in calves, and latency can persist following the decline in colostral immunity, with calves remaining seronegative (Homan & Easterday 1983). If the infection is initiated via the oral cavity, nasal cavity, or ocular orifices, the primary sites for latency are the sensory neurons within trigeminal ganglia (TG). Relatively high levels of viral gene expression (Schang & Jones 1997) or infectious virus (Inman et al. 2002) can be detected in TG within 1 6 days after infection. A hallmark of latency is the abundant level of transcription that occurs from the latency-related (LR) gene (Jones 1998, 2003; Jones et al. 2006) and open reading frame-e (ORF-E) (Inman et al. 2004). ORF-E is at the downstream of the gene, encoding the major viral transcriptional activator bicp0. After acute infection, some factors help in the establishment of latency, i.e., LR gene, ORF-E, neuronal factor, and cell-mediated immunity (CMI) response in TG (Jones and Chowdhury 2008). LR gene products induce latency by inhibiting apoptosis of virus-infected cells (Ciacci-Zanella et al. 1999; Henderson et al. 2004) and viral gene expression (Bratanich et al. 1992; Geiser et al. 2002). ORF-E may have a role in the establishment of latency because it can induce neuritelike outgrowth in mouse neuroblastoma cells (Perez et al. 2007). Consequently, ORF-E may be responsible for restoration of mature neuronal functions following the infection. Neuronal factors inhibit productive infection and CMI response in TG. It leads to abundant viral transcripts, viral protein, and viral DNA replication (Feldman et al. 2002), inducing latent infection. Maintenance of latent infection is mostly controlled by LR gene and ORF-E. LR gene inhibits bicp0 RNA expression, which is a viral promoter, and ORF-E maintains the neural health (Jones & Chowdhury 2008). The cattle that are seronegative for BHV-1 antibodies may be latently infected with BHV-1 (Hage et al. 1997). Latency may also occur in non-neural sites such as tonsillar lymphoid cells (Winkler et al. 2000), peripheral blood (Fuchs et al. 1999), and lymphnodes (Mweene et al. 1996). 3. BHV-1-related diseases BHV-1 or infectious bovine rhinotracheitis (IBR) virus is an important causative agent of respiratory infection, abortion, conjunctival infection, and other respiratorytract diseases. The clinical manifestation of BHV-1 infection is dependent on the nature of various subtypes. BHV-1 causes three different types of infection, namely respiratory infection (BHV-1.1), genital infection (BHV- 1.2), and neurological disease (BHV-1.3). The respiratory infection is characterized by high fever, mucopurulent nasal discharge, and excessive salivation. The laesion

6 72 S. Biswas et al. includes rhinotracheitis, pharyngitis, and laryngotracheitis (Gibbs & Rweyemanu 1977; Yates 1982). The virus with co-infection of some bacteria might induce severe bronchopneumonia, pleuritis, thoracic pain, and audible rubbing. In genital infection, there is development of pustules, ulcers in the mucosa of vulva and vagina with frequent urination. Abortion occurs at the end of the fifth month of pregnancy, with expulsion of dead foetus and blood stained fluids. The nervous manifestation of this viral infection is mostly seen as a form of encephalitis in calves, with the virus presumed to have spread from nasal mucosa through trigeminal ganglion. The virus remains latent in trigeminal ganglion and sacral ganglion for several time periods. BHV-1 often causes enteritis in calves due to replication in the digestive tract. (BVDV), parainfluenza-3 virus or bovine respiratory syncytial virus, and the bacteria Mannheimia haemolytica or Pasteurella multocida (Yates 1982). BHV-1 can initiate BRDC by causing immunosuppression (Winkler et al. 1999; Lovato et al. 2003), allowing secondary infections that lead to severe pneumonia and death (Hanon et al. 1998; Lovato et al. 2003). BRDC is a serious pneumonic condition that affects up to 50% of cattle in Australia, causing death of upto 5% of all the cattle (Meat & Livestock Australia 2001), costing the Australian feedlot industry around $60 million each year (CSIRO 2005). Control of bovine respiratory disease can be possible only with an increased understanding of both the respiratory and immune systems of the cow and of the interaction of the host, pathogen, and environment Clinical course In BHV-1 infection, after an incubation period of 2 4 days, serous nasal discharge, salivation, fever, anorexia, and depression become evident. Within a few days the nasal and ocular discharges become mucopurulent. Where natural mating is practised, genital infection can lead to pustular vulvovaginitis or balanoposthitis. However, most infections run a very mild or subclinical course (van Oirschot et al. 1993). An uncomplicated case of respiratory or genital disease caused by BHV-1 usually lasts for about 5 10 days. Secondary bacterial or viral agents may contribute to a multifactor disease complex resulting in severe respiratory diseases in young animals ( shipping or crowding fever ). After infection via the airborne route, BHV-1 replicates in high numbers in mucous membranes of the upper respiratory tract and tonsils. Subsequently, the virus disseminates to conjunctivae and reaches the trigeminal ganglia by neuro-axonal transport. After genital infection, BHV-1 replicates in the mucous membranes of the vagina or prepuce and becomes latent in the sacral ganglia. Viral DNA remains in the neurons of the ganglia, probably for the entire life of the host. The reactivation of the latent infection can be due to stressful conditions such as transport and parturition, and also due to the application of corticosteroids (Muylkens et al. 2007). Consequently, the virus may switch between latent and lytic infection, and may be shed intermittently into the environment and spread to in-contact animals Bovine respiratory disease complex The Bovine Respiratory Disease Complex (BRDC) consists of at least three clinical entities, as well as several additional diseases which affect the respiratory tract secondarily or as part of a more generalized disease. The three clinical entities are as follows: (1) enzootic pneumonia of calves, (2) shipping fever complex, and (3) atypical interstitial pneumonia. BHV-1 is one of the agents that cause BRDC. During shipment, cattle may be subjected to crowded conditions, exhaustion, irregular feeding and watering, climatic changes, and sick cattle. BRDC results from a combination of stress and infectious agents, in particular the viruses BHV-1, bovine viral diarrhoea virus 3.3. Pathogenesis, pathophysiology, and signalling pathway After entry into the body, replication occurs at the portal of entry or within the nasal or genital mucosa. During the initial replication at the portal of entry, the herpesviruses may enter the axons of local nerve cells. Then, by intraaxonal transport, the viruses reach the neuron bodies in the regional ganglia where latency can be established (Nandi et al. 2009). Transmission into the body is achieved through blood, nerves, and infected tissues via cell-to-cell interaction. Following transient viraemia, secondary sites will be infected, such as the digestive tract, udder, foetus, and ovaries. From the site of infection, peripheral nerves are reached by retrograde axonal transportation, i.e., trigeminal ganglion in case of respiratory infection, and sacral ganglion after genital infection. Viral entry into cells is a multistep process involving several glycoproteins and at least two cellular receptors (Mettenleiter 1994). Glycoprotein gc of alphaherpesviruses initiates these steps by binding to heparan sulphate proteoglycans on the cell surface. The binding of gc to heparan sulfate moieties leads to a loose attachment that is followed by fixed binding of gd to the putative second cellular receptor. Binding of gd is necessary for initiation of viral entry (Karger et al. 1995), and for steps between virus binding and membrane fusion by interacting with other cellular or viral components. Viral entry into the cell is finally mediated by fusion of the viral envelope with the cell membrane, due to interactions of gb, gh, and gl (Liang et al. 1995). Nyaga and McKercher (1980) have shown by in vitro examinations that BHV-1 can infect blood monocytes, where a limited virus replication and release is possible. In addition, BHV-1 is able to absorb to lymphocytes which may also serve as vehicles, at least as long as no neutralizing antibodies are present. The virus multiplies in the respiratory tract and causes inflammatory changes such as rhinitis, laryngitis, and tracheitis, leading to destruction of the tracheal microvilli. Infection of the cattle with BHV-1 impairs resistance to secondary bacterial infections such as M. haemolytica, P. multocida, and H. somni, leading to depression of cellmediated immunity and subsequent fatality (Yates 1982; Leite et al. 2002). Laesions may extend from the nasal

7 Veterinary Quarterly 73 tract to the eyes through the nasolacrymal duct, and may give rise to conjunctivitis and nasal discharge. In yaks, BHV-1 infection is mostly associated with Moraxella bovis-, M. haemolytica-, and Neisseria-associated keratoconjunctivitis (Bandyopadhyay et al. 2010a, 2010b). The virus may enter the brain tissues from the nasal mucosa via the trigeminal nerves causing meningoencephalitis. The virus might also cause changes in the placenta and foetus, resulting in abortion. 4. Epidemiology The first infection of BHV-1 was recorded in the form of genital disease as infectious pustular vulvo-vaginitis (IPV) in cattle in 1841 by Buchner & Trommsdrof in Germany. Viral association with this disease was first demonstrated in 1928 by Reisinger & Reimann. In the 1950s, emergence of the respiratory form of the disease as IBR was observed in North America. In 1958, the virus was isolated successfully for the first time and its antigenic identity was revealed. Later this viral agent was classified under the family of Herpesviridae. BHV-1 is currently widespread all over the world and reported for instance in USA, Canada, Zaire, Italy, Belgium, India, and Turkey (Castrucci et al. 1997; Bilgedagalap 1998; Boelaert et al. 2000; Yesilbag et al. 2003; Rajkhowa et al. 2004). Serological surveys in the cattle, carried out in Turkey, ascertained that this virus is widespread among the dairy and beef cattle in many regions of the country (Cabalar & Akca 1994; Alkan et al. 2000; Aly et al. 2003; Akca et al. 2004). Previous research by Cabalar and Can-Sahna (2000) revealed that the seropositivity rate of BHV-1 was between 20% and 74% in the cattle. BHV-1 especially infects domestic and wild cattle, and other ruminants may be similarly infected (International terrestial ). In previous studies, cross-species infections by bovine and caprine herpesviruses were demonstrated (Lehmkuhl et al. 1985; Yesilbag et al. 2003). Detection of antibodies against BHV-1 in sheep suggests that sheep may play a crucial role in the epidemiology and maintenance of BHV-1 in the environment (Elazhary et al. 1984; Jetteur et al. 1990). However, sheep is unlikely to play any role in BHV-1 transmission (Hage et al. 1997). In the UK, the prevalence of BHV-1 has increased to 83% in unvaccinated herds (Woodbine et al. 2009). Control programs are ongoing in several other countries, like in Germany and Italy (OIE 2010). The seroprevalence of BHV-1 has been reported to be 14% 60% in Africa and 36% 48% in Central and South America (Straub 1990), 36% in China (Yan et al. 2008), 43% in England (Woodbine et al. 2009), and 63% 86% in Eygpt (Mahmoud et al. 2009). Several European countries successfully implemented the IBR eradication program. Countries like Austria, Denmark, Finland, Sweden, and Switzerland are officially free of IBR (Ackermann & Engels 2005). Like other countries, India was also affected by this disease as the virus was detected in many parts of the country, like Kerala (Sulochana et al. 1982), Gujarat (Singh et al. 1983), Tamil Nadu (Manickam & Mohan 1987), Orissa, Arunachal Pradesh (Bandyopadhyay et al. 2009), Nagaland (Rajkhowa et al. 2004), and Karnataka (Mohan Kumar et al. 1994). Given a grave concern regarding exotic bovine species like mithun and yak, the association with BHV was determined. The seroprevalence of IBR in yak is highest over the age of 3 years and lowest in the first year of life. The gender or the location of the yaks (farm or free ranging) was not a factor influencing the prevalence of the virus. The overall seroprevalence in yak was found to be 41% by virus neutralization test (VNT) and avidin biotin enzyme-linked immunosorbent assay (AB-ELISA). The virus was also detected in the ocular swab of yaks suffering from infectious bovine keratoconjunctivitis (Bandyopadhyay et al. 2009; Bandyopadhyay et al. 2010a). The origin and geographic distribution of BHV-5 infection is largely unknown mainly due to its serological cross-reactivity with BHV-1 (Vogel et al. 2002). Sporadic cases of meningoencephalitis due to BHV-5 have been reported in Australia (Johnston et al. 1962), USA (Eugster et al. 1974), Italy (Moretti et al. 1964), and Hungary (Bartha et al. 1969). In contrast, BHV-5 infection and disease appear to be more frequent in Argentina and Brazil, where numerous outbreaks were described in the last decades (Carrillo et al. 1983; Weiblen et al. 1989; Roehe et al. 1997; Rissi et al. 2006). The rare occurrence of BHV-5 neurological disease in areas where BHV-1 infection is endemic may be explained by cross-protection induced by natural infection or vaccination (Thiry et al. 2006). 5. Immune response to BHV-1 infection The immune response of cattle to BHV-1 infection is unique. While there are similarities in immune responses to other alphaherpesviruses, the bovine response to BHV-1 is not identical to that of herpes simplex virus in mice or in humans, and does not correlate precisely with experimental BHV-1 infection in mice (Babiuk et al. 1996). The immune response to BHV-1 infection is triggered when the virus begins to replicate (Babiuk et al. 1996). Adaptive cell-mediated and antibody-mediated immune response occurs 7 days after infection (Engels & Ackermann 1996). Antibody response is thought to be critical in preventing infection and viral spread, while cell-mediated immunity is involved in recovery from infection (Babiuk et al. 1996) Humoral response Experimental as well as natural infection and vaccination demonstrated that the antibodies are triggered against the gb, gc, gd, and ge glycoproteins (Tikoo et al. 1995a), protecting against viremia and associated severe disease (Mechor et al. 1987). The antibody response includes mostly neutralizing antibodies, and contributes to antiviral antibody-dependent cellular cytotoxicity (Tikoo et al. 1995a), which is often complement mediated (Rouse et al. 1977). Antibodies in the circulation may be recorded for an endurable period, like 3 years following BHV-1 vaccination (Hage et al. 1997). In contrast, the antibody response to the V155 strain of BHV-1 persists at maximal levels from 7 to 21 days after infection (Bagust 1972). Maternal antibody to BHV-1 persists for 123 days after

8 74 S. Biswas et al. weaning at 2 months of age (Fulton et al. 2003). Newborn calves are protected from BHV-1 infection after being fed colostrum collected from vaccinated cows (Mechor et al. 1987), although maternal antibody is not completely protective since calves can have latent BHV-1 infections early in life in the presence of maternal antibody too (SCAHW 2000). stimulation (Forman et al. 1982). The effect of immunosuppression is partly mediated by the BHV-1 gg glycoprotein, a broad-spectrum chemokine-binding protein that blocks chemokine binding and activity (Bryant et al. 2003). BHV-1 also infects CD4þ T cells, inducing a loss of CD4 expression followed by apoptosis of these cells (Winkler et al. 1999; Lovato et al. 2003) Cell-mediated immune response The cell-mediated immune response to BHV-1 infection is under the control of macrophages, interleukin-2, and interferon-g production, natural killer cells and natural killer-like activity, proliferation of viral gc- and gdspecific CD4þ T-cells, and stimulation of cytotoxic T- lymphocyte activity (Hutchings et al. 1990; Tikoo et al. 1995b). Interferon-g, interferon-a, and interferon-b have been shown to both protect against infection and to prevent viral spread in experimental infection in mice (Abril et al. 2004). Responses to BHV-1 infection are broad based and include both T helper cell 1 and T helper cell 2 responses (Babiuk et al. 1996), although, as with other intracellular pathogens, there is a skew towards a T helper cell 1-type response (Mena et al. 2002) Allergenicity There are no reports of BHV-1 encoding known allergens or causing an allergic response Immune-evasion, immune-modulation, and immunosuppression BHV-1 evades the host immune response by interfering with MHC-mediated antigen processing and presentation following infection of monocytes and macrophages (Nyaga & McKercher 1980; Forman et al. 1982). Alphaherpesviruses, including BHV-1, also have immunomodulatory activity mediated by herpesvirus proteins that mimic key molecules of the host immune system (Raftery et al. 2000). For example, these viruses express proteins that bind complement C3 in a species-specific manner and thus alter the host immune response to allow viral infection (Huemer et al. 1993; Engels & Ackermann 1996). Additionally, latency is also established by immune evasion. During latency, viral proteins are not expressed and infection occurs at immunoprivileged sites that do not express major histocompatibility class I antigens (Tyler & Nathanson 2001). BHV-1 was also reported to cause immunosuppression in infected cattle, which often leads to secondary viral and bacterial infections (Winkler et al. 1999) contributing to BRDC. Immunosuppression is caused by impairment of macrophage, polymorphonuclear neutrophil, and lymphocyte function (Tikoo et al. 1995a), and by decreased IL-2 receptor expression, decreased mitogenic stimulation of peripheral blood mononuclear cells, and reduced numbers of circulating T lymphocytes (Winkler et al. 1999). Infection of monocytes and macrophages leads to impaired phagocytosis, reduced antibodydependent cellular cytotoxicity function, and poor T cell 5.5. Immunity and relation to stress Immunity to BHV-1 occurs mostly due to either natural infection or vaccination (Denis et al. 1994; Tikoo et al. 1995a). Immunity involves both cellular and humoral response to various glycoproteins (Babiuk et al. 1996). There are some factors facilitating elimination of infection from the body such as natural antibodies preventing the attachment of virus to cells and interaction with complement in order to lyse the cells infected by the virus. Monocytes or polymorphonuclear cells can also trigger the lysis of the infected cells with the aid of F c -receptors. There are several glycoproteins promoting attachment and penetration of virus into cells, i.e., gb, gc, and gd. These glycoproteins also help in intercellular transmission of virus. After establishment of infection, early cytokines are released, i.e., interferon-a, TNF, interleukin-1, within a few hours and maximum levels are reached after 36 hours. Interferon-a recruits leukocytes at the sites of infection (Bielefeldt et al. 1991; Griebel et al. 1989; Griebel et al. 1998). Pro-inflammatory cytokines are released by epithelial cells and alveolar macrophages, leading to expression of adhesion molecules which retain leukocytes at the site of infection (Bochner et al. 1987; Lamontagne et al. 1985). This phenomenon causes increased vascular permeability and adhesion between cells leading to generation of reactive oxygen species (ROS), arachidonic acid, and other factors that prevent virus replication and promote killing of infected cells by different mechanisms. Killing of infected cells may also occur in the absence of antibody by natural killer cells and macrophages (Campos et al. 1994; Campos et al. 1989; Campos & Rossi 1986; Palmer et al. 1990). T-cells help in activation of macrophages regarding killing the BHV-infected cells by secretion of interferon-g (Campos et al. 1989). In addition, macrophages and natural-killer (NK) cells produce cytokines that influence the development of specific immune responses. Activation of T-helper cells I and II (Th1/Th2) generate the production of other cytokines which improve T and B cell responses. Both antibody and cell-mediated immunity are important factors in ameliorating the disease. Elevated corticosteroid levels (due to stress) and/or immune suppression can initiate reactivation from latency. The stress associated with moving cattle from one location to another is one obvious stimulus that can trigger reactivation from latency and induction of BRDC. This reactivation from latency was also recorded in yaks following extreme stress like prolonged transportation in the mountainous tracts and severe nutritional deprivation as seen in harsh winter season (Bandyopadhyay et al. 2007). Interestingly, deficiency of important trace minerals like zinc and copper which are directly associated with intracellular

9 Veterinary Quarterly 75 oxidant/antioxidant defence mechanism and immune status was recorded to have higher correlation with BHV-1 infection in yaks as evidenced by higher seropositivity (Bandyopadhyay et al. 2007; Bandyopadhyay et al. 2009; Bandyopadhyay et al. 2010b). During reactivation from latency, three significant events occur: 1) productive viral gene expression is readily detected in sensory neurons, 2) both the ORF-E and LR gene expression decrease dramatically, and 3) infective virus is secreted from nasal or ocular swabs (Jones 1998, 2003; Jones et al. 2006). Administration of dexamethasone to calves or rabbits, latently infected with BHV-1, reproducibly leads to activation of viral gene expression and reactivation from latency (Rock et al. 1992; Jones 1998, 2003; Jones et al. 2000, 2006; Inman et al. 2002). The ability of dexamethasone to induce apoptosis of inflammatory cells in TG of calves latently infected with BHV-1 correlates well with reactivation from latency (Winkler et al. 2002). In yaks also, molecular detection of BHV-1 in the nasal discharge was possible following prednisolone or dexamethasone administration suggesting increased virus secretion from nasal discharge (Bandyopadhyay et al. 2007). Varying virus titers ranging from 103 to 106 TCID 50 ml 1 (tissueculture infective dose) during reactivation and reexcretion have been reported after stress (Pastoret et al. 1982; Straub 1990), transport (Thiry et al. 1987), infection with parainfluenza-3 (PI-3) virus (Mensik et al. 1976) or Dictyocaulus viviparous (Msolla et al. 1983), parturition, treatment with dexamethasone and adrenocorticotropic hormone (ACTH), and uptake of 3-methylindole. Spontaneous reactivation without clinical signs has also been observed at irregular intervals (Schultz et al. 1977; Grom et al. 2006). 6. Impact over livestock industry Introduction of IBR into a cattle farm can cause severe economic losses due to weight loss, decrease in milk production, and restrictions in the international livestock trade (Nandi et al. 2009). Cattle recovering from IBR infection are very prone to become a silent carrier. These animals remain carriers of BHV-1 for the rest of their life and immunosuppressive treatments or conditions might reactivate virus replication, leading to spread of the infection to the rest of the herd (Van Oirschot 1997; Preston & Nicholl 2008). The same is true for rare bovine species like the yak and mithun. The yak (Bos grunniens) is a bovine species of high economic importance, living in the hills and snowbound areas at m above the mean sea level in China, Mongolia, Bhutan, Nepal, Russia, and India (Weiner et al. 1994; Bandyopadhyay et al. 2009). They are mostly reared for milk, meat, and wool. The products obtained from the yak are considered to be organic due their geographical locations that are free from environmental pollutants (Bandyopadhyay et al. 2007). BHV-1 infection causes a sharp drop in milk production with loss of body weight, abortion, and decreased show value of animals due to bilateral conjunctivitis, chemosis, and extreme restlessness (Bandyopadhyay et al. 2010a). The mithun (Bos frontalis) is a ruminant species found in the hilly regions of northeast India, Myanmar, Bhutan, Bangladesh, China, and Malaysia (Rajkhowa et al. 2004). It is a source of meat and milk. Milk of mithun contains a higher amount of protein, fat, and solids-non-fat than that of buffalo but less lactose (Rajkhowa et al. 2004). Bovine rhinotracheitis causes a huge loss of productivity in mithun as well, and infection is prevalent in all varieties of mithun, namely the races of AP (39%), Mizoram (18%), and Nagaland (15%), according to Rajkhowa et al. (2004). 7. Diagnosis BHV infection can be diagnosed by cell culture, histopathology, serology, PCR, and electron microscopy Cell culture BHV-1 can be readily isolated in cell culture of primary or secondary bovine kidney, lungs, testis, turbinate, or trachea and established cell lines such as Madin Darby Bovine Kidney (MDBK) or CRIB cells (Flores & Donis 1995; Nandi et al. 2009). The virus can be isolated from nasal swabs, conjunctival swabs, vaginal swabs, preputial washing, placental cotyledons of aborted foetus, fetal liver, lung, spleen, kidney, lymph node, mucous membrane of the respiratory tract, tonsils, and lungs collected in virus transport medium. The presence of virus in specimens is detected by a cytopathic effect (CPE). The CPE of BHV-1 is characteristic and usually appears within 3 days of inoculation. There are grape-like clusters of rounded cells present around a microplaque in cell culture. Giant cells or syncytia are also observed. The virus is cytolytic if the cells are incubated for a prolonged time and there is total sloughing of the rounded cells from the plastic/glass surface of the container. The cell cultures inoculated with specimens are observed for 7 days. The cell culture should be passaged at least three times before the sample is considered negative (Straub 1990; Turin and Russo 2003) Histopathology Intranuclear viral inclusions of Cowdry type A can occasionally be identified in the epithelial cells of vaginal biopsy tissues collected in the early stage of IPV but not in cells collected in nasal discharge of cattle with IBR (Nandi et al. 2009). These inclusions are also present in the brain from cases of encephalitis, and in tissues of aborted foetuses. As these inclusions are transitory, the use of histological examination for diagnosis is of limited value (Turin & Russo 2003). Perivascular cuffing with neuronophagia, satellitosis, haemorrhage, and neuronal degeneration are seen in encephalitic form of BHV infection (Bagust & Cleark 1972; Belknap et al. 1994; Meyer et al. 2001; Perez et al. 2003) Electron microscopy The use of electron microscopy to identify virus particles in clinical material is a rapid method for the diagnosis of

10 76 S. Biswas et al. BHV-1 but it should be used in the early stage of the disease (Nandi et al. 2009) Serology Several serological tests are available for the detection of antibody and a rise in titre between the acute and convalescent phase of infection. The primary immune response to BHV-1 experimental inoculation of cattle is characterized by the formation of both IgM and IgG antibodies. Secondary immune responses are characterized primarily by the formation of IgG 2 antibody. The VNT has been widely used and is the gold standard by which other techniques have been evaluated (Perrin et al. 1996). However, the ELISA is a specific, sensitive, and more practical test for detection of BHV-1 antibodies. A variety of ELISAs, namely indirect ELISA, c-elisa, and AB-ELISA have been employed to screen serum samples of cattle and buffaloes in India (Nandi et al. 2004, 2007). The IgM-ELISA is useful for the diagnosis of recent infection with BHV-1 in calves (Ungar-Waron & Abraham 1991). Furthermore, a micro-elisa is being used for the control program of BHV-1 infection in Switzerland. The test is simple, rapid, and convenient compared to the serum neutralization test, which requires cell culture facilities and is time-consuming. The only currently available assay that differentiates antibodies against BHV-1 from BHV-5 is a BHV-1 ge blocking ELISA (Wellenberg et al. 2001). Of note, an antibody- ELISA and VNT were successfully employed in yaks and mithuns also (Rajkhowa et al. 2004; Bandyopadhyay et al. 2009) 7.5. PCR The PCR assay is as sensitive as virus isolation and is a practical alternative for the rapid detection of virus. The results are available in 1 day compared to virus isolation which requires 7 days. Virus could be detected in nasal swabs for upto 14 days after experimental infection of the cattle and the PCR assay can also detect the virus in bovine fetal serum and semen samples. The PCR assay is considered equivalent to that of standard virus isolation and dot blot hybridization (Xia et al. 1995). The PCR assay with southern blot hybridization is considered to be highly sensitive and can detect the virus in semen before detectable antibody development (Masri et al. 1996). Real-time PCR provides satisfactory reproducibility as well as high specificity and sensitivity in combination with significant reduction in time for detecting amplified products (Nandi et al. 2009). In order to differentiate between BHV-1 and BHV-5, several assays are available like nested PCR (Ashbaugh et al. 1997), multiplex PCR (Alegre et al. 2001; Claus et al. 2005) and multiple PCR sequencing assay (Del Medico Zajac 2007). Of interest, a highly sensitive nested PCR was reported to detect glycoprotein B and glycoprotein E of the virus in biological samples from yaks (Bandyopadhyay et al. 2010a). 8. Vaccination With currently available diagnostic tests, it is not possible to identify animals which have a latent BHV-1 infection. The next best strategy is to use a well-planned vaccination program. Different types of vaccine are available, namely modified live virus (MLV) vaccines, inactivated vaccines, subunit vaccines, and marker vaccines Modified live virus vaccines There are three types of MLV vaccine available. The parenteral vaccine is made from bovine fetal kidney tissue culture. Besides, there are two intranasal vaccines available either of rabbit tissue culture origin or of bovine tissue culture origin, containing the mutant form of BHV-1 (Nandi et al. 2009). The MLV vaccines offer a rapid immune response concomitant with relatively long-lasting local mucosal immunity (Whetstone et al. 1986). Both parenteral and intranasal vaccines stimulate the production of humoral antibody. The intranasal vaccine stimulates the production of local interferon and local antibody in the nasal mucosa and is safe for use in pregnant cows. Furthermore, it is highly effective in the prevention of abortion. Intranasal vaccines provide protection against respiratory form within 72 hours of administration. For intranasal vaccination, 2 ml of diluents containing vaccine should be administered in one nostril carefully because this vaccine only multiplies in the nasal mucosa. After intranasal vaccination, virus is shed for 7 14 days, with peak shedding occurring at 4 days. The parenteral MLV vaccine is potentially abortigenic and should not be used in non-immune pregnant animals. It is of importance to realize that the virus from MLV vaccine sometimes becomes latent following administration Inactivated vaccines The inactivated vaccines have some advantages over MLV vaccines because they do not cause abortion, immunosuppression, or latency. However, they do not fully prevent latency by field strains. Usually two doses are administered at an interval of days and protection is observed 7 10 days following the second dose (Patel 2005). Inactivated vaccines are not as efficacious as MLV vaccines because of potential destruction of some of the protective antigens during the inactivation process by alkylating agents. To improve efficacy, an adjuvant is always added (Johannes et al. 2004) Subunit vaccine A subunit vaccine contains one or more of the antigens of the virus necessary to evoke protective immunity, and lacks nucleic acid and other components that might cause unwanted side effects (Brunner et al. 1988). In BHV-1, gb, gc, and gd glycoproteins are immunogenic, and are separated from the virus-infected cells or the peptide is synthesized (Nandi et al. 2009). Calves are vaccinated in between 3 7 months of age with booster after 12 days of

11 Veterinary Quarterly 77 primary vaccination. The level of immunity based on serum antibody titres and protection against experimental challenge is much greater with individual glycoproteins than those immunized with commercially available inactivated vaccine. Another subunit BHV-1 vaccine containing only gd glycoprotein along with recombinant M. haemolytica vaccine was reported to be superior to MLV BHV-1 vaccine in reducing mortality due to respiratory disease (Nandi et al. 2009). It does not contain live virus, so there is no chance to cause abortion or establish the latent infection. Furthermore, there is potentiality to differentiate between vaccinated and naturally infected animals. However, its efficacy depends upon the adjuvant used and sufficient amount of glycoprotein required to induce immunity. The subunit vaccine was considered superior to the MLV BHV-1 vaccine in reducing mortality due to respiratory disease (Nandi et al. 2009) Marker vaccine Marker vaccine is based on deletion of one or more viral proteins, which allows the distinction between vaccinated and naturally infected animals based upon respective antibody responses (Oirschot et al. 1996). Different types of marker vaccines are available like ge-live, ge-killed, ggkilled, gc-live, gd-subunit, gb-subunit, and gdreplication-incompetent. Calves vaccinated at the age of 7 weeks showed reduction both in clinical signs and excretion of challenge virus as early as 7 days after IM injection or 3 days after intranasal vaccination. Antibodies against marker vaccine were detectable in milk within 2 3 weeks and persisted in the body more than 2 3 years if not probably lifelong. The ge-negative marker vaccines, live as well as killed, are already used in control or eradication programs in the EU (European Union 2000) Multivalent vaccine Multivalent vaccine is available for the control of coinfection associated with BHV-1. These vaccines contain other respiratory pathogens such as parainfluenza-3 (PI-3), bovine respiratory syncytial virus (BRSV) and bovine viral diarrhoea virus (BVDV). Sometimes it also contains antigens of Leptospira and Campylobacter sp. A combination vaccine containing ge-negative live vaccine, BRSV, and PI-3, administered at 2 and 6 weeks of age, has been shown to be effective in that it reduced severity of clinical signs and the amount of virus shedding after experimental challenge infection (Mars et al. 2000). The vaccination of calves with multivalent vaccines containing MLV or MLV and inactivated BHV-1 is associated with virus-specific interferon gamma production and protection from clinical disease due to challenge, 5 days after a single vaccination (Campos et al. 1989; Patel 2005; Nandi et al. 2009). 9. Conclusion In a nutshell, BHV-1 is an emerging concern which has the potentiality to cripple the livestock industry. The diagnostic tools are time consuming and expensive. The available prophylactic strategies have their own limitations to develop a holistic control program against this transboundary pathogen. In-depth research with practical and implementable outcome is necessary to effectively tackle this pathogen which is slowly but deceptively spreading among our livestock population. 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