ABSTRACT
Snakehead vesiculovirus (SHVV) has caused mass mortality to cultured snakehead fish in China, resulting in enormous economic losses in snakehead fish culture. In this report, the whole genome of SHVV was sequenced. Interestingly, it shared more than 94% nucleotide sequence identity with Monopterus albus rhabdovirus (MoARV), which has caused great economic loss to cultured rice field eel (Monopterus albus). Therefore, the concern of cross-species infection of these viruses prompted us to investigate the susceptibility of rice field eel to SHVV infection. The results showed that rice field eel was susceptible to SHVV in both intracoelomical injection and immersion routes. Severe hemorrhage was observed on the skin and visceral organs of SHVV-infected rice field eels. Histopathological examination showed vacuoles in the tissues of infected liver, kidney and heart. Viral RNA or protein was detected in the tissues of infected fish by reverse transcription polymerization chain reaction (RT-PCR), in situ hybridization (ISH), or immunohistochemistry assay (IHC). Investigation of the epidemic of vesiculovirus in rice field eel as well as other co-cultured fish is invaluable for the prevention of vesiculovirus infection.
Subject(s)
Eels/virology , Fish Diseases/pathology , Fish Diseases/virology , Rhabdoviridae Infections/veterinary , Vesiculovirus/pathogenicity , Animal Structures/pathology , Animal Structures/virology , Animals , China , Computational Biology , Histocytochemistry , Immunohistochemistry , In Situ Hybridization , RNA, Viral/analysis , Reverse Transcriptase Polymerase Chain Reaction , Rhabdoviridae Infections/pathology , Rhabdoviridae Infections/virology , Sequence Homology, Nucleic Acid , Vesiculovirus/genetics , Vesiculovirus/isolation & purification , Viral Proteins/analysis , Whole Genome SequencingABSTRACT
Chandipura virus (CHPV) has been contributing to the rising number of premature deaths due to acute encephalitis syndrome for over a decade in India. CHPV belongs to the family Rhabdoviridae. Neuropathogenesis of CHPV has been well established but the exact route of entry into the central nervous system (CNS) and the triggering factor for neuronal death are still unknown. Rabies virus and vesicular stomatitis virus, which are related closely to CHPV, enter the CNS retrogradely from peripheral or olfactory neurons. Disruption of the blood-brain barrier has also been connoted in the entry of CHPV into the CNS. CHPV upon entering the neurons triggers cellular stress factors and release of reactive oxygen species (ROS). The stress granules produced in response to cellular stress have been implicated in viral replication and ROS generation, which stimulates neuronal death. Both these phenomena cohesively explain the neuropathogenesis and neurodegeneration following CHPV infection.
Subject(s)
Acute Febrile Encephalopathy/epidemiology , Endemic Diseases/statistics & numerical data , Rhabdoviridae Infections/epidemiology , Vesiculovirus/pathogenicity , Zoonoses/epidemiology , Acute Febrile Encephalopathy/prevention & control , Acute Febrile Encephalopathy/virology , Animals , Endemic Diseases/prevention & control , Humans , India/epidemiology , Mosquito Vectors/virology , Psychodidae/virology , Rhabdoviridae Infections/prevention & control , Rhabdoviridae Infections/transmission , Rhabdoviridae Infections/virology , Vesiculovirus/isolation & purification , Vesiculovirus/physiology , Zoonoses/prevention & control , Zoonoses/transmission , Zoonoses/virologyABSTRACT
Piry virus (PIRYV) is a rhabdovirus (genus Vesiculovirus) and is described as a possible human pathogen, originally isolated from a Philander opossum trapped in Para State, Northern Brazil. This study describes the complete full coding sequence and the genetic characterization of PIRYV. The genome sequence reveals that PIRYV has a typical vesiculovirus-like organization, encoding the five genes typical of the genus. Phylogenetic analysis confirmed that PIRYV is most closely related to Perinet virus and clustered in the same clade as Chandipura and Isfahan vesiculoviruses.
Subject(s)
Genome, Viral , Vesiculovirus/genetics , Base Sequence , Genomics , Humans , Molecular Sequence Data , Phylogeny , RNA, Viral/genetics , Rhabdoviridae Infections/virology , Vesiculovirus/classification , Vesiculovirus/isolation & purification , Viral Proteins/geneticsABSTRACT
Here, we describe the use of DNA-conjugated antibodies for rapid and sensitive detection of whole viruses using a single-particle interferometric reflectance imaging sensor (SP-IRIS), a simple, label-free biosensor capable of imaging individual nanoparticles. First, we characterize the elevation of the antibodies conjugated to a DNA sequence on a three-dimensional (3-D) polymeric surface using a fluorescence axial localization technique, spectral self-interference fluorescence microscopy (SSFM). Our results indicate that using DNA linkers results in significant elevation of the antibodies on the 3-D polymeric surface. We subsequently show the specific detection of pseudotyped vesicular stomatitis virus (VSV) as a model virus on SP-IRIS platform. We demonstrate that DNA-conjugated antibodies improve the capture efficiency by achieving the maximal virus capture for an antibody density as low as 0.72 ng/mm(2), whereas for unmodified antibody, the optimal virus capture requires six times greater antibody density on the sensor surface. We also show that using DNA conjugated anti-EBOV GP (Ebola virus glycoprotein) improves the sensitivity of EBOV-GP carrying VSV detection compared to directly immobilized antibodies. Furthermore, utilizing a DNA surface for conversion to an antibody array offers an easier manufacturing process by replacing the antibody printing step with DNA printing. The DNA-directed immobilization technique also has the added advantages of programmable sensor surface generation based on the need and resistance to high temperatures required for microfluidic device fabrication. These capabilities improve the existing SP-IRIS technology, resulting in a more robust and versatile platform, ideal for point-of-care diagnostics applications.
Subject(s)
Antibodies, Immobilized/chemistry , Biosensing Techniques , DNA Probes/chemistry , DNA/chemistry , Vesiculovirus/isolation & purification , Biosensing Techniques/instrumentation , Microscopy, Fluorescence/instrumentation , Vesiculovirus/pathogenicityABSTRACT
BACKGROUND: The sudden death of 10 children in a tribal village of Kandhamal district, Odisha in eastern India led to this investigation. METHODS: We conducted a door-to-door survey to identify cases. Antibodies for Chandipura, Japanese encephalitis, dengue, chikungunya and West Nile viruses were tested by ELISA in probable cases. Chandipura virus RNA was tested from both human blood samples and sand flies by reverse transcriptase polymerase chain reaction. We conducted vector surveys in domestic and peridomestic areas, and collected sand flies. RESULTS: Entomological investigations revealed the presence of Phlebotomus argentipes and Sergentomiya sp. Thirty-five patients presented with fever, 12 of them had altered sensorium including 4 who had convulsions. The blood samples of 21 patients were tested; four samples revealed Chandipura virusspecific IgM antibody. CONCLUSION: Chandipura virus infection causing encephalitis affected this tribal population in eastern India at 1212 m above sea level.
Subject(s)
Chikungunya Fever , Disease Outbreaks , Encephalitis, Viral , Phlebotomus/virology , Vesiculovirus , Adolescent , Adult , Animals , Antibodies, Viral/analysis , Chikungunya Fever/blood , Chikungunya Fever/complications , Chikungunya Fever/diagnosis , Chikungunya Fever/epidemiology , Chikungunya Fever/physiopathology , Child , Disease Vectors , Encephalitis, Viral/blood , Encephalitis, Viral/diagnosis , Encephalitis, Viral/etiology , Encephalitis, Viral/mortality , Encephalitis, Viral/physiopathology , Female , Humans , Immunoglobulin M/blood , India/epidemiology , Male , RNA, Viral/blood , Vesiculovirus/isolation & purification , Vesiculovirus/pathogenicityABSTRACT
BACKGROUND & OBJECTIVES: An outbreak of acute encephalitis syndrome was reported from Vidarbha region of Maharashtra s0 tate, India, during July 2012. Anti-IgM antibodies against Chandipura virus (CHPV) were detected in clinical samples. Sandfly collections were done to determine their role in CHPV transmission. METHODS: Twenty nine pools of Sergentomyia spp. comprising 625 specimens were processed for virus isolation in Vero E6 cell line. Diagnostic RT-PCR targeting N-gene was carried out with the sample that showed cytopathic effects (CPE). The PCR product was sequenced, analysed and the sequences were deposited in Genbank database. RESULTS: CPE in Vero E6 cell line infected with three pools was detected at 48 h post infection. However, virus could be isolated only from one pool. RT-PCR studies demonstrated 527 nucleotide product that confirmed the agent as CHPV. Sequence analysis of the new isolate showed difference in 10-12 nucleotides in comparison to earlier isolates. INTERPRETATION & CONCLUSIONS: This is perhaps the first isolation of CHPV from Sergentomyia spp. in India and virus isolation during transmission season suggests their probable role in CHPV transmission. Further studies need to be done to confirm the precise role of Sargentomyia spp. in CHPV transmission.
Subject(s)
Phlebotomus/pathogenicity , Psychodidae/virology , Rhabdoviridae Infections/transmission , Vesiculovirus/isolation & purification , Animals , Antibodies, Anti-Idiotypic/isolation & purification , Chlorocebus aethiops , Encephalitis/epidemiology , Encephalitis/virology , India , Phlebotomus/virology , Psychodidae/pathogenicity , Rhabdoviridae Infections/epidemiology , Rhabdoviridae Infections/virology , Vero Cells , Vesiculovirus/pathogenicityABSTRACT
BACKGROUND: Malpais Spring virus (MSPV) is a mosquito-borne rhabdovirus that infects a variety of wild and feral ungulates in New Mexico, including horses and deer. Although, initial serologic tests and electron microscopy at the time of isolation nearly 25 years ago provided evidence that MSPV is a novel virus, possibly related to vesiculoviruses, the virus still has not been approved as a new species. FINDINGS: Use of the illumina platform allowed us to obtain the complete genome of MSPV. Analysis of the complete 11019 nt genome sequence of the prototype 85-488NM strain of MSPV indicates that it encodes the five common rhabdovirus structural proteins (N, P, M, G and L) with alternative ORFs (> 180 nt) in the N, M and G genes, including a 249 nt ORF in the G gene predicted to encode a 9.26 kDa highly basic transmembrane protein. Although antigenically very distant, phylogenetic analysis of the L gene indicates that MSPV is most closely related to Jurona virus, also isolated from mosquitoes in Brazil, as well as a number of other vesiculoviruses. CONCLUSIONS: In sum, our analysis indicates MSPV should be classified as a member of the genus Vesiculovirus, family Rhabdoviridae. The complete genome sequence of MSPV will be helpful in the development of a reverse genetics system to study the unique aspects of this vesiculovirus in vivo and in vitro, and will assist development of specific diagnostic tests to study the epidemiology of MSPV infection.
Subject(s)
Genome, Viral , RNA, Viral/genetics , Sequence Analysis, DNA , Vesiculovirus/classification , Vesiculovirus/genetics , Animals , Cluster Analysis , Molecular Sequence Data , Open Reading Frames , Phylogeny , Vesiculovirus/isolation & purification , Viral Proteins/geneticsABSTRACT
The complete coding sequences were determined for four putative vesiculoviruses isolated from fish. Sequence alignment and phylogenetic analysis based on the predicted amino acid sequences of the five main proteins assigned tench rhabdovirus and grass carp rhabdovirus together with spring viraemia of carp and pike fry rhabdovirus to a lineage that was distinct from the mammalian vesiculoviruses. Perch rhabdovirus, eel virus European X, lake trout rhabdovirus 903/87 and sea trout virus were placed in a second lineage that was also distinct from the recognised genera in the family Rhabdoviridae. Establishment of two new rhabdovirus genera, "Perhabdovirus" and "Sprivivirus", is discussed.
Subject(s)
Fish Diseases/virology , Fishes/virology , Genome, Viral , Rhabdoviridae Infections/veterinary , Vesiculovirus/classification , Vesiculovirus/genetics , Animals , Carps/virology , Cyprinidae/virology , Eels/virology , Fishes/classification , Perches/virology , Phylogeny , RNA, Viral/genetics , Rhabdoviridae Infections/virology , Sequence Analysis, DNA , Vesiculovirus/isolation & purificationABSTRACT
We present pyrosequencing data and phylogenetic analysis for the full genome of Yug Bogdanovac virus (YBV), a member of the Vesicular stomatitis virus serogroup of the Rhabdoviridae isolated from a pool of Phlebotomus perfiliewi sandflies collected in Serbia in 1976. YBV shows very low nucleotide identities to other members of the Vesicular stomatitis virus serogroup and does not contain a reading frame for C'/C proteins.
Subject(s)
Genome, Viral , RNA, Viral/genetics , Sequence Analysis, DNA , Vesiculovirus/genetics , Animals , Cluster Analysis , Molecular Sequence Data , Phlebotomus/virology , Phylogeny , Sequence Homology , Serbia , Vesiculovirus/isolation & purificationABSTRACT
Spring viraemia of carp (SVC) is a viral disease that mainly affects carp Cyprinus carpio and other cyprinid fish, causing severe economic losses. Rapid detection and identification of spring viraemia of carp virus (SVCV) is crucial for effective disease management. Recent advances in nanoscience are having a significant impact on many scientific fields, especially biodiagnostics, where a number of nanoparticle-based assays have been introduced for biomolecular detection. Single- and double-stranded oligonucleotides can be adsorbed on gold nanoparticles (AuNPs) in colloidal solution under certain conditions. We exploited this phenomenon to develop a specific hybridization assay for direct detection of SVCV-RNA without prior amplification. The result of the hybridization process could be detected visually within 1 min when the colour of the reaction mixture changed from red to blue (positive reaction) or remains red (negative). The lower detection limit of the assay was estimated to be 10-3 TCID50 ml-1 SVCV-RNA, and it has the feasibility to detect the target virus-RNA in clinical specimens without previous amplification. In order to obtain an indication of the assay's performance on clinical samples we compared the optimized assay with nested RT-PCR in detection of SVCV-RNA in infected fish samples. The concordance of the 2 methods was defined as 100% when compared to nested RT-PCR positive and negative samples. The SVC-AuNPs assay requires only 15 min, eliminates the need for thermal cycling or detection instruments and is a specific and rapid tool for detection of SVCV-RNA directly from clinical samples.
Subject(s)
Carps/virology , Gold/chemistry , Metal Nanoparticles/chemistry , RNA, Viral/isolation & purification , Rhabdoviridae Infections/veterinary , Vesiculovirus/isolation & purification , Animals , Colorimetry/methods , Colorimetry/veterinary , Fish Diseases/virology , Rhabdoviridae Infections/diagnosis , Sensitivity and Specificity , Viral Envelope Proteins/geneticsABSTRACT
Vesicular stomatitis virus (VSV) has long been regarded as a promising recombinant vaccine platform and oncolytic agent but has not yet been tested in humans because it causes encephalomyelitis in rodents and primates. Recent studies have shown that specific tropisms of several viruses could be eliminated by engineering microRNA target sequences into their genomes, thereby inhibiting spread in tissues expressing cognate microRNAs. We therefore sought to determine whether microRNA targets could be engineered into VSV to ameliorate its neuropathogenicity. Using a panel of recombinant VSVs incorporating microRNA target sequences corresponding to neuron-specific or control microRNAs (in forward and reverse orientations), we tested viral replication kinetics in cell lines treated with microRNA mimics, neurotoxicity after direct intracerebral inoculation in mice, and antitumor efficacy. Compared to picornaviruses and adenoviruses, the engineered VSVs were relatively resistant to microRNA-mediated inhibition, but neurotoxicity could nevertheless be ameliorated significantly using this approach, without compromise to antitumor efficacy. Neurotoxicity was most profoundly reduced in a virus carrying four tandem copies of a neuronal mir125 target sequence inserted in the 3'-untranslated region of the viral polymerase (L) gene.
Subject(s)
Encephalitis, Viral/therapy , MicroRNAs/genetics , Vesiculovirus/isolation & purification , Animals , Base Sequence , Cell Line , Cricetinae , DNA Primers , Down-Regulation/genetics , Encephalitis, Viral/virology , Humans , Lethal Dose 50 , Mice , Mice, SCID , Polymerase Chain Reaction , Vesiculovirus/pathogenicity , Vesiculovirus/physiology , Virus ReplicationABSTRACT
Vesicular stomatitis (VS) viruses have been classified into two serotypes: New Jersey (VSNJV) and Indiana (VSIV). Here, we have characterized field isolates causing vesicular stomatitis in Brazil and Argentina over a 35-year span. Cluster analysis based on either serological relatedness, as inferred from virus neutralization and complement fixation assays, or nucleotide sequences of two separate genes (phosphoprotein or glycoprotein) grouped the field isolates into two distinct monophyletic groups within the Indiana serogroup. One group included seven viruses from Brazil and Argentina that were serologically classified as Indiana-2 and Cocal virus (COCV). The other group contained three viruses from Brazil that were serologically classified as Indiana-3 and the prototype of this group, Alagoas virus (VSAV). Interestingly, two vesiculoviruses that were isolated from insects but do not cause disease in animals, one from Brazil (Maraba virus; MARAV) and the other from Colombia (CoAr 171638), grouped into two separate genetic lineages within the Indiana serotype. Our data provide support for the classification of viruses causing clinical VS in livestock in Brazil and Argentina into two distinct groups: Indiana-2 (VSIV-2) and Indiana-3 (VSIV-3). We suggest using nomenclature for these viruses that includes the serotype, year and place of occurrence, and affected host. This nomenclature is consistent with that currently utilized to describe field isolates of VSNJV or VSIV in scientific literature.
Subject(s)
Antigens, Viral/immunology , Cattle Diseases/virology , Horse Diseases/virology , Insecta/virology , Rhabdoviridae Infections/veterinary , Vesiculovirus/genetics , Vesiculovirus/immunology , Animals , Antigens, Viral/genetics , Cattle , Horses , Molecular Sequence Data , Neutralization Tests , Phylogeny , Rhabdoviridae Infections/virology , South America , Vesiculovirus/classification , Vesiculovirus/isolation & purificationABSTRACT
An improvement to a previously reported real-time reverse transcription polymerase chain reaction (real-time RT-PCR) assay for the detection of Vesicular stomatitis virus (VSV) is described. Results indicate that the new assay is capable of detecting a panel of genetically representative strains of VSV present in North, Central, and South America. The assay is specific for VSV and allows for simultaneous differentiation between Vesicular stomatitis Indiana virus and Vesicular stomatitis New Jersey virus. This real-time RT-PCR is able to detect current circulating strains of VSV and can be used for rapid diagnosis of VSV and differentiation of VSV from other vesicular diseases, such as foot-and-mouth disease.
Subject(s)
Reverse Transcriptase Polymerase Chain Reaction/methods , Vesicular Stomatitis/epidemiology , Vesicular stomatitis Indiana virus/genetics , Vesicular stomatitis New Jersey virus/genetics , Vesiculovirus/genetics , Animals , Base Pair Mismatch , Base Sequence , Central America/epidemiology , DNA Primers , DNA Probes , Gene Amplification , Mexico/epidemiology , Reverse Transcriptase Polymerase Chain Reaction/standards , Sequence Homology, Nucleic Acid , South America/epidemiology , United States/epidemiology , Vesicular stomatitis Indiana virus/classification , Vesicular stomatitis Indiana virus/isolation & purification , Vesicular stomatitis New Jersey virus/classification , Vesicular stomatitis New Jersey virus/isolation & purification , Vesiculovirus/classification , Vesiculovirus/isolation & purificationABSTRACT
We report on a supramolecular sensor array using fluorogenic peptide probes and graphene oxide that can target glycoproteins on a viral caspid, facilitating the differentiation of ebola virus from marburg virus and receptor-extensive vesicular stomatitis virus using principal component analysis.
Subject(s)
Biosensing Techniques , Capsid Proteins/chemistry , Ebolavirus/isolation & purification , Fluorescent Dyes/chemistry , Glycoproteins/chemistry , Graphite/chemistry , Peptides/chemistry , Marburgvirus/isolation & purification , Vesiculovirus/isolation & purificationABSTRACT
Knowledge of the many mechanisms of vesicular stomatitis virus (VSV) transmission is critical for understanding of the epidemiology of sporadic disease outbreaks in the western United States. Migratory grasshoppers [Melanoplus sanguinipes (Fabricius)] have been implicated as reservoirs and mechanical vectors of VSV. The grasshopper-cattle-grasshopper transmission cycle is based on the assumptions that (i) virus shed from clinically infected animals would contaminate pasture plants and remain infectious on plant surfaces and (ii) grasshoppers would become infected by eating the virus-contaminated plants. Our objectives were to determine the stability of VSV on common plant species of U.S. Northern Plains rangelands and to assess the potential of these plant species as a source of virus for grasshoppers. Fourteen plant species were exposed to VSV and assayed for infectious virus over time (0 to 24 h). The frequency of viable virus recovery at 24 h postexposure was as high as 73%. The two most common plant species in Northern Plains rangelands (western wheatgrass [Pascopyrum smithii] and needle and thread [Hesperostipa comata]) were fed to groups of grasshoppers. At 3 weeks postfeeding, the grasshopper infection rate was 44 to 50%. Exposure of VSV to a commonly used grasshopper pesticide resulted in complete viral inactivation. This is the first report demonstrating the stability of VSV on rangeland plant surfaces, and it suggests that a significant window of opportunity exists for grasshoppers to ingest VSV from contaminated plants. The use of grasshopper pesticides on pastures would decrease the incidence of a virus-amplifying mechanical vector and might also decontaminate pastures, thereby decreasing the inter- and intraherd spread of VSV.
Subject(s)
Grasshoppers/virology , Plants/virology , Vesiculovirus/isolation & purification , Animals , Eating , Microbial Viability , Rhabdoviridae Infections/transmission , Time Factors , United StatesABSTRACT
Definitive diagnosis of vesicular or vesicular-like lesions in livestock animals presents challenges both for veterinary clinicians and diagnostic laboratories. It is often impossible to diagnose the causative disease agent on a clinical basis alone and difficult to collect ample vesicular epithelium samples. Due to restrictions of time and sample size, once laboratory tests have ruled out foot-and-mouth disease, vesicular stomatitis and swine vesicular disease a definitive diagnosis may remain elusive. With the ability to test a small quantity of sample for a large number of pathogens simultaneously, DNA microarrays represent a potential solution to this problem. This study describes the application of a long oligonucleotide microarray assay to the identification of viruses known to cause vesicular or vesicular-like lesions in livestock animals. Eighteen virus isolates from cell culture were successfully identified to genus level, including representatives of each foot-and-mouth disease virus serotype, two species of vesicular stomatitis virus (VSV), swine vesicular disease virus, vesicular exanthema of swine virus (VESV), bovine herpesvirus 1, orf virus, pseudocowpox virus, bluetongue virus serotype 1 and bovine viral diarrhoea virus 1. VSV and VESV were also identified in vesicular epithelium samples, with varying levels of sensitivity. The results indicate that with further development this microarray assay could be a valuable tool for the diagnosis of vesicular and vesicular-like diseases.
Subject(s)
Cattle Diseases/diagnosis , Foot-and-Mouth Disease/diagnosis , Oligonucleotide Array Sequence Analysis/veterinary , Swine Diseases/diagnosis , Swine Vesicular Disease/diagnosis , Vesicular Stomatitis/diagnosis , Animals , Cattle , Cattle Diseases/virology , DNA, Viral/chemistry , DNA, Viral/genetics , Female , Foot-and-Mouth Disease/pathology , Foot-and-Mouth Disease/virology , Foot-and-Mouth Disease Virus/isolation & purification , Oligonucleotide Array Sequence Analysis/methods , RNA, Viral/chemistry , RNA, Viral/genetics , Sensitivity and Specificity , Swine , Swine Diseases/pathology , Swine Diseases/virology , Swine Vesicular Disease/pathology , Swine Vesicular Disease/virology , Vesicular Stomatitis/pathology , Vesicular Stomatitis/virology , Vesiculovirus/isolation & purificationABSTRACT
Host factor requirements for different classes of viruses have not been fully unraveled. Replication of the viral genome and synthesis of viral proteins within the human host cell are associated with an increased demand for nutrients and specific metabolites. With more than 400 acknowledged members to date in humans, solute carriers (SLCs) represent the largest family of transmembrane proteins dedicated to the transport of ions and small molecules such as amino acids, sugars and nucleotides. Consistent with their impact on cellular metabolism, several SLCs have been implicated as host factors affecting the viral life cycle and the cellular response to infection. In this study, we aimed at characterizing the role of host SLCs in cell survival upon viral infection by performing unbiased genetic screens using a focused CRISPR knockout library. Genetic screens with the cytolytic vesicular stomatitis virus (VSV) showed that the loss of two SLCs genes, encoding the sialic acid transporter SLC35A1/CST and the zinc transporter SLC30A1/ZnT1, affected cell survival upon infection. Further characterization of these genes suggests a role for both of these transporters in the apoptotic response induced by VSV, offering new insights into the cellular response to oncolytic virus infections.
Subject(s)
Carcinoma, Non-Small-Cell Lung/pathology , Cation Transport Proteins/metabolism , Lung Neoplasms/pathology , Nucleotide Transport Proteins/metabolism , Rhabdoviridae Infections/complications , Virus Replication , Carcinoma, Non-Small-Cell Lung/genetics , Carcinoma, Non-Small-Cell Lung/metabolism , Carcinoma, Non-Small-Cell Lung/virology , Cation Transport Proteins/genetics , Genetic Engineering , Host-Pathogen Interactions , Humans , Lung Neoplasms/genetics , Lung Neoplasms/metabolism , Lung Neoplasms/virology , Nucleotide Transport Proteins/genetics , Rhabdoviridae Infections/virology , Tumor Cells, Cultured , Vesiculovirus/isolation & purificationABSTRACT
Spring viremia of carp virus (SVCV), infectious hematopoietic necrosis virus (IHNV) and viral hemorrhagic septicemia virus (VHSV) are three important fish rhabdoviruses, causing serious Office International des Epizooties (OIE) classified diseases in wild and farmed fish. Here, a new multiplex real-time quantitative RT-PCR (mqRT-PCR) assay was developed for simultaneous detection, identification and quantification of these three rhabdoviruses. The sets of primers and probes were targeted to conserved regions of glycoprotein (G) gene of SVCV, nucleoprotein (N) gene of IHNV and G gene of VHSV and used to amplify. The sensitivity, specificity and interference test of mqRT-PCR assay was analyzed. It was shown that the detection levels of 100 copies of SVCV, 220 copies of IHNV and 140 copies of VHSV were achieved, and there was no non-specific amplification and cross-reactivity using RNA of pike fry rhabdovirus (PFRV), infectious pancreatic necrosis virus (IPNV) and grass carp reovirus (GCRV). A total of 80 clinical fish samples were tested using the mqRT-PCR assay and the results were confirmed by antigen-capture ELISA and cell culture assay. This assay has the potential to be used for both research applications and diagnosis.
Subject(s)
Infectious hematopoietic necrosis virus/isolation & purification , Novirhabdovirus/isolation & purification , Reverse Transcriptase Polymerase Chain Reaction/methods , Vesiculovirus/isolation & purification , Animals , Cell Line , Fish Diseases/diagnosis , Fish Diseases/virology , Fishes/virology , Rhabdoviridae Infections/diagnosis , Rhabdoviridae Infections/veterinary , Rhabdoviridae Infections/virology , Sensitivity and SpecificityABSTRACT
A highly sensitive and specific one-step multiplex RT-PCR assay has been developed and standardised for the simultaneous and differential detection of the most important vesicular viruses affecting livestock: foot-and-mouth disease virus (FMDV), swine vesicular disease virus (SVDV), and vesicular stomatitis virus (VSV). The method uses three primer sets, each one specific for the corresponding virus, selected to detect of all serotypes of FMD and VS. The detection range was confirmed by examination of a collection of 31 isolates of the three target viruses. The specificity of the assay was also demonstrated by testing other related viruses, uninfected cell line cultures and healthy pig tissues. The testing of blood and serum samples from animals infected experimentally proved that the method can be useful for early diagnosis of the diseases, even before the first vesicular lesions are visualized in the infected pigs. An assessment of the performance of the multiplex RT-PCR was carried out using a panel of more than 100 samples from animals infected experimentally, showing the suitability of the method for a rapid (less than 6h), sensitive and specific differential diagnosis in clinical samples. Additionally, a uniplex RT-PCR for VSV, that amplifies the two viral serotypes, was also developed and tested as a rapid tool for the diagnosis of this vesicular disease.
Subject(s)
Enterovirus B, Human/isolation & purification , Foot-and-Mouth Disease Virus/isolation & purification , Foot-and-Mouth Disease/diagnosis , Reverse Transcriptase Polymerase Chain Reaction/methods , Swine Vesicular Disease/diagnosis , Vesicular Stomatitis/virology , Vesiculovirus/isolation & purification , Animals , Diagnosis, Differential , Foot-and-Mouth Disease/virology , Sensitivity and Specificity , Swine , Swine Diseases/diagnosis , Swine Diseases/virology , Swine Vesicular Disease/virologyABSTRACT
BACKGROUND: Chandipura virus (CHPV), a member of family Rhabdoviridae was attributed to an explosive outbreak of acute encephalitis in children in Andhra Pradesh, India in 2003 and a small outbreak among tribal children from Gujarat, Western India in 2004. The case-fatality rate ranged from 55-75%. Considering the rapid progression of the disease and high mortality, a highly sensitive method for quantifying CHPV RNA by real-time one step reverse transcriptase PCR (real-time one step RT-PCR) using TaqMan technology was developed for rapid diagnosis. METHODS: Primers and probe for P gene were designed and used to standardize real-time one step RT-PCR assay for CHPV RNA quantitation. Standard RNA was prepared by PCR amplification, TA cloning and run off transcription. The optimized real-time one step RT-PCR assay was compared with the diagnostic nested RT-PCR and different virus isolation systems [in vivo (mice) in ovo (eggs), in vitro (Vero E6, PS, RD and Sand fly cell line)] for the detection of CHPV. Sensitivity and specificity of real-time one step RT-PCR assay was evaluated with diagnostic nested RT-PCR, which is considered as a gold standard. RESULTS: Real-time one step RT-PCR was optimized using in vitro transcribed (IVT) RNA. Standard curve showed linear relationship for wide range of 102-1010 (r2 = 0.99) with maximum Coefficient of variation (CV = 5.91%) for IVT RNA. The newly developed real-time RT-PCR was at par with nested RT-PCR in sensitivity and superior to cell lines and other living systems (embryonated eggs and infant mice) used for the isolation of the virus. Detection limit of real-time one step RT-PCR and nested RT-PCR was found to be 1.2 x 100 PFU/ml. RD cells, sand fly cells, infant mice, and embryonated eggs showed almost equal sensitivity (1.2 x 102 PFU/ml). Vero and PS cell-lines (1.2 x 103 PFU/ml) were least sensitive to CHPV infection. Specificity of the assay was found to be 100% when RNA from other viruses or healthy individual was used. CONCLUSION: On account of the high sensitivity, reproducibility and specificity, the assay can be used for the rapid detection and quantitation of CHPV RNA from clinical samples during epidemics and from endemic areas. The assay may also find application in screening of antiviral compounds, understanding of pathogenesis as well as evaluation of vaccine.