1.Serosurveillance for Japanese encephalitis virus infection among equines in India.
Baldev R GULATI ; Harisankar SINGHA ; Birendra K SINGH ; Nitin VIRMANI ; Sandip K KHURANA ; Raj K SINGH
Journal of Veterinary Science 2011;12(4):341-345
The seroprevalence of Japanese encephalitis virus (JEV) among equines was evaluated from January 2006 to December 2009 in 13 different states of India by hemagglutination inhibition (HI) test and virus neutralization test (VNT). Antibodies against JEV were detected in 327 out of 3,286 (10%) equines with a maximum prevalence reported in the state of Manipur (91.7%) followed by Gujarat (18.5%), Madhya Pradesh (14.4%), and Uttar Pradesh (11.6%). Evidence of JEV infection was observed in equines in Indore (Madhya Pradesh) where a 4-fold or higher rise in antibody titer was observed in 21 out of 34 horses in November 2007 to October 2006. In March 2008, seven of these horses had a subsequent 4-fold rise in JEV antibody titers while this titer decreased in nine animals. JEV-positive horse sera had a JEV/WNV (West Nile virus) ratio over 2.0 according to the HI and/or VNT. These results indicated that JEV is endemic among equines in India.
Animals
;
Encephalitis, Japanese/blood/epidemiology/*veterinary
;
*Equidae
;
India/epidemiology
;
Neutralization Tests
;
Seroepidemiologic Studies
;
Time Factors
2.Isolation and genetic characterization of Japanese encephalitis virus from equines in India.
Baldev R GULATI ; Harisankar SINGHA ; Birendra K SINGH ; Nitin VIRMANI ; Sanjay KUMAR ; Raj K SINGH
Journal of Veterinary Science 2012;13(2):111-118
Japanese encephalitis (JE) is an important vector-borne viral disease of humans and horses in Asia. JE outbreaks occur regularly amongst humans in certain parts of India and sporadic cases occur among horses. In this study, JE seroprevalence and evidence of JE virus (JEV) infection among horses in Haryana (India) is described. Antibodies against JEV were detected in 67 out of 637 (10.5%) horses screened between 2006 and 2010. Two foals exhibiting neurological signs were positive for JEV RNA by RT-PCR; JEV was isolated from the serum of one of the foals collected on the second day of illness. This is the first report of JEV isolation from a horse in India. Furthermore, a pool of mosquitoes collected from the premises housing these foals was positive for JEV RNA by RT-PCR. Three structural genes, capsid (C), premembrane (prM), and envelope (E) of the isolated virus (JE/eq/India/H225/2009) spanning 2,500 nucleotides (from 134 to 2,633) were cloned and sequenced. BLAST results showed that these genes had a greater than 97% nucleotide sequence identity with different human JEV isolates from India. Phylogenetic analysis based on E- and C/prM genes indicated that the equine JEV isolate belonged to genotype III and was closely related to the Vellore group of JEV isolates from India.
Animals
;
Antibodies, Monoclonal
;
Cloning, Molecular
;
Culex/virology
;
Encephalitis Virus, Japanese/*genetics/*isolation & purification
;
Encephalitis, Japanese/epidemiology/*veterinary/virology
;
Enzyme-Linked Immunosorbent Assay/methods/veterinary
;
Female
;
Genes, Viral
;
Genotype
;
Horse Diseases/epidemiology/*virology
;
Horses
;
India/epidemiology
;
RNA, Viral/genetics/isolation & purification
;
Reverse Transcriptase Polymerase Chain Reaction/veterinary
;
Seroepidemiologic Studies