Your search keyword '"bovine ephemeral fever virus"' showing total 17 results

1. Production of Monoclonal Antibody against Prokaryotically Expressed G1 Protein of Bovine Ephemeral Fever Virus.

Author

Pasandideh, R., Shapouri, M. R. Seyfi Abad, and Nassiri, M. T. Beigi

Subjects

*MONOCLONAL antibodies, *THREE-day sickness in cattle, *PROTEIN expression, *VIRAL proteins, *ENZYME-linked immunosorbent assay

Abstract

Epitope-G1 of bovine ephemeral fever virus (BEFV) G glycoprotein has been genetically and antigenically conserved among various isolates of BEFV and only reacts with anti-BEFV neutralising antibodies. Therefore, it is a candidate antigen for development of the enzyme linked immunosorbent assay (ELISA) for serological identification bovine ephemeral fever (BEF)-infected animals. The aim of this study was to produce a monoclonal antibody (MAb) against recombinant G1 antigen expressed into Escherichia coli. For this purpose, somatic cell hybrids between SP2/0 myeloma cells and spleen cells derived from Balb/c mice immunized with maltose-binding protein (MBP)-G1 fusion protein were established. After three rounds of cloning, the stability of antibody secretion in the positive clones was confirmed by ELISA and the reactivity of the MAbs against recombinant G1 was verified by Western blot analysis. The specific MAbs produced against recombinant G1 antigen in this study could be used for establishing BEFV diagnostic experiments in the future. [ABSTRACT FROM AUTHOR]

Published

2019

2. Molecular characterization of bovine ephemeral fever virus in Thailand between 2013 and 2017.

Author

Chaisirirat, Thanawat, Sangthong, Pradit, Arunvipas, Pipat, Petcharat, Nantawan, Thangthamniyom, Nattarat, Chumsing, Wilairat, and Lekcharoensuk, Porntippa

Subjects

*THREE-day sickness in cattle, *CATTLE infections, *GENETIC code, *NUCLEOTIDES, *VETERINARY epidemiology

Abstract

Highlights • This is the first report on genetics of bovine ephemeral fever virus (BEFV) in Southeast Asia and the connection of BEFV circulation in Asia. • Thai BEFVs were divided into two clusters in the second and third sub-clades of East Asia lineage. • BEFVs that caused high motility rate in cattle are in the third sub-clade. • P' ORF of Thai BEFV contains a premature stop codon resulting in a shorter ORF of 64 instead of 147 nucleotides. • The complete genome of Thai (LRI0045) and Chinese (J02L) BEFVs share several common characteristics. Abstract Bovine ephemeral fever (BEF) is an arthropod-borne disease caused by bovine ephemeral fever virus (BEFV), a negative sense, single-stranded RNA virus. BEFV is endemic in tropical and sub-tropical regions including Thailand, a country in mainland Southeast Asia. However, there are few studies on BEFV and no available information regarding molecular characteristics of BEFV in Thailand. Therefore, the aims of this study were to genetically characterize Thai BEFVs and reveal their evolutions by phylogenetic analysis of G gene ectodomain sequences. From 2013 to 2017, blood samples were collected from bovine that matched with BEF case definition from three regions of Thailand. Thai BEFV G genes and a whole genome of an isolate, East Asia/TH/LRI0045/2016, were sequenced and characterized. Additionally, their phylogenies were constructed. This is the first report on genetics of BEFV in Southeast Asia. G ectodomain encoding region of Thai BEFV found during 2013–2017 are closely related to the second and third sub-clades of East Asia lineage. In addition, we observed mutation in the putative P' ORF of all Thai BEFVs which generated a premature stop codon. Thai G gene sequences are closely related to those of mainland Chinese and Taiwanese isolates. The whole genomic sequences of Thai BEFV and East Asia/China/JT02 L/2002 possess common characteristics, suggesting shared evolutionary relationship between East and Southeast Asian strains. Further studies on relationship between animal translocation, circulation of BEFV in Greater Mekong subregion and acquisition of more G gene sequences may improve understanding of BEFV epidemiology in mainland Southeast Asia. [ABSTRACT FROM AUTHOR]

Published

2018

3. High-resolution melting (HRM) for genotyping bovine ephemeral fever virus (BEFV).

Author

Erster, Oran, Stram, Rotem, Menasherow, Shopia, Rubistein-Giuni, Marisol, Sharir, Binyamin, Kchinich, Evgeni, and Stram, Yehuda

Subjects

*THREE-day sickness in cattle, *VIRAL genomes, *NUCLEOTIDE sequence, *EPIDEMICS, *TOPSIS method

Abstract

In recent years there have been several major outbreaks of bovine ephemeral disease in the Middle East, including Israel. Such occurrences raise the need for quick identification of the viruses responsible for the outbreaks, in order to rapidly identify the entry of viruses that do not belong to the Middle-East BEFV lineage. This challenge was met by the development of a high-resolution melt (HRM) assay. The assay is based on the viral G gene sequence and generation of an algorithm that calculates and evaluates the GC content of various fragments. The algorithm was designed to scan 50- to 200-base-long segments in a sliding-window manner, compare and rank them using an Order of Technique of Preference by Similarity to Ideal Solution (TOPSIS) the technique for order preference by similarity to ideal solution technique, according to the differences in GC content of homologous fragments. Two fragments were selected, based on a match to the analysis criteria, in terms of size and GC content. These fragments were successfully used in the analysis to differentiate between different virus lineages, thus facilitating assignment of the viruses’ geographical origins. Moreover, the assay could be used for differentiating infected from vaccinated animales (DIVA). The new algorithm may therefore be useful for development of improved genotyping studies for other viruses and possibly other microorganisms. [ABSTRACT FROM AUTHOR]

Published

2017

4. Post-viraemic detection of bovine ephemeral fever virus by use of autogenous lymphoid tissue-derived bovine primary cell cultures.

Author

Barigye, R, Davis, S, Hunt, R, Hunt, N, Walsh, S, Elliott, N, Dyrting, K, Weir, R, and Melville, LF

Subjects

*THREE-day sickness in cattle, *CATTLE infections, *LYMPHOID tissue, *REVERSE transcriptase polymerase chain reaction, *NEUTROPHILS, *PHYSIOLOGY

Abstract

Background The potential tissue replication sites and specific cell types that support in vivo virus survival beyond the acute phase of bovine ephemeral fever virus ( BEFV) infection have not been fully defined in cattle. To clarify the knowledge gap, tissue specimens were tested after collection from an adult steer necropsied 1 week after acute BEF. Case report Significant necropsy findings included fibrinoproliferative synovitis in the stifle joints and fibrin clot-laden fluid in serous body cavities. Moderate numbers of infiltrating neutrophils were demonstrated in sections of the prefemoral lymph nodes and haemal node, and lymphoid hyperplasia in the spleen, haemal node and prefemoral lymph nodes. Viral RNA was detected by qRT-PCR in fresh spleen, haemal node, prefemoral lymph node, synovial fluid and in several spleen-derived cell cultures. BEFV was isolated from autogenously derived splenic primary cell cultures 6 days after cessation of viraemia, and characteristic bullet-shaped virions were confirmed by electron microscopy of an ultrathin haemal node section. In sections of the spleen, haemal node and other tissues, immunohistochemistry demonstrated BEFV antigens that were intracellularly associated with probable histiocytic cells. Conclusion BEFV has preferential tropism for bovine lymphoid tissues and the spleen and haemal node may be potential sites for post-viraemic virus replication. [ABSTRACT FROM AUTHOR]

Published

2017

5. Viral neurotropism, peripheral neuropathy and other morphological abnormalities in bovine ephemeral fever virus-infected downer cattle.

Author

Barigye, R, Davis, S, Hunt, R, Hunt, N, Walsh, S, Elliott, N, Burnup, C, Aumann, S, Day, C, Dyrting, K, Weir, R, and Melville, LF

Subjects

*PERIPHERAL neuropathy, *THREE-day sickness in cattle, *NEURODEGENERATION, *ENCEPHALITIS, *COW diseases

Abstract

Objective This study assessed the neurotropism of bovine ephemeral fever (BEF) virus (BEFV) and described histomorphological abnormalities of the brain, spinal cord and peripheral nerves that may causally contribute to paresis or paralysis in BEF. Methods Four paralysed and six asymptomatic but virusinfected cattle were monitored, and blood and serum samples screened by qRT-PCR, virus isolation and neutralisation tests. Fresh brain, spinal cord, peripheral nerve and other tissues were qRT-PCR-tested for viral RNA, while formalin-fixed specimens were processed routinely and immunohistochemically evaluated for histomorphological abnormalities and viral antigen distribution, respectively. Results The neurotropism of BEFV was immunohistochemically confirmed in the brain and peripheral nerves and peripheral neuropathy was demonstrated in three paralysed but not the six aneurological but virus-infected animals. Wallerian degeneration (WD) was present in the ventral funicular white matter of the lumbar spinal cord of a paralysed steer and in cervical and thoracic spinal cord segments of three paralysed animals. Although no spinal cord lesions were seen in the steer euthanased within 7 days of illness, peripheral neuropathy was present and more severe in nerves of the brachial plexuses than in the gluteal or fibular nerves. The only steer with WD in the lumbar spinal cord also showed intrahistiocytic cell viral antigen that was spatially distributed within areas of moderate brain stem encephalitis. Conclusion The data confirmed neurotropism of BEFV in cattle and documented histomorphological abnormalities in peripheral nerves and brain which, together with spinal cord lesions, may contribute to chronic paralysis in BEFV-infected downer cattle. [ABSTRACT FROM AUTHOR]

Published

2016

6. New genetic mechanism, origin and population dynamic of bovine ephemeral fever virus.

Author

He, Cheng-Qiang, Liu, Ya-Xin, Wang, Hong-Mei, Hou, Pei-Li, He, Hong-Bin, and Ding, Nai-Zheng

Subjects

*THREE-day sickness in cattle, *POPULATION dynamics, *EPIDEMICS, *PHYLOGEOGRAPHY, *RHABDOVIRUSES

Abstract

Bovine ephemeral fever virus (BEFV) is a typical species of the genus Ephemerovirus in the family Rhabdoviridae. Today, prevailing BEFV can be divided into three phylogeographic lineages, East Asia, Mideast, and Australia. In this study, we provide evidence that the whole East Asia lineage originates from a homologous recombination (HR) between the Mideast and Australia lineages that probably occurred in the 1940s. To our knowledge, HR has not been proposed before as the genetic mechanism of BEFV. According to the HR event and Bayesian estimation, the three BEFV lineages might originate from Africa, and may have spread to Asia and Australia through the Mideast. In addition, the population of the virus may have augmented significantly in the 2000s, suggesting that the risk for outbreaks of BEFV may be high at present. [ABSTRACT FROM AUTHOR]

Published

2016

7. The geographical distribution and first molecular analysis of Culicoides Latreille (Diptera: Ceratopogonidae) species in the Southern and Southeastern Turkey during the 2012 outbreak of bovine ephemeral fever.

Author

Dik, B., Muz, D., Muz, M., and Uslu, U.

Subjects

*CERATOPOGONIDAE, *MOLECULES, *THREE-day sickness in cattle, *NUCLEIC acids

Abstract

This study investigated the geographical distribution and molecular analysis of Culicoides species in the Southern and Southeastern Turkey during the 2012 outbreak of bovine ephemeral fever (BEF). The midge specimens caught by Onderstepoort-type light traps from livestock farms were tested for molecular evidence of existence of viral genome. Blood specimens were collected from clinically BEF-suspected acute febrile cattle. Total nucleic acid samples obtained from field specimens were checked against the BEF virus G gene and Culicoides internal transcribed spacer 1 (ITS-1) gene. A total of 20,845 Culicoides specimens (20,569 ♀♀, 276 ♂♂) comprising 11 species ( Culicoides badooshensis, Culicoides circumscriptus, Culicoides gejgelensis, Culicoides imicola, Culicoides kibunensis, Culicoides longipennis, Culicoides newsteadi, Culicoides nubeculosus, Culicoides odiatus, Culicoides punctatus, Culicoides schultzei, Culicoides spp.) were collected. C. schultzei (18,032) was found as the dominant species and followed by C. imicola (1,857), C. nubeculosus complex (545), and C. circumscriptus (259), respectively. C. kibunensis was identified as new species for this region. PCR positivity of BEF was found 37.14 % (13/35) in blood samples whereas no viral genome was obtained from Culicoides specimens. Culicoides spp. ITS-1 gene sequences were analyzed phylogenetically with GenBank ITS-1 sequences. Molecular homology of Culicoides ITS-1 gene was ranged between 62.74 and 71.39 %. The results described first molecular detection and phylogenetic analysis of Culicoides ITS-1 gene with reference to the 2012 BEF outbreak in Turkey. [ABSTRACT FROM AUTHOR]

Published

2014

8. A Large-Scale Outbreak of Bovine Ephemeral Fever in Turkey, 2012.

Author

TONBAK, Sukru, BERBER, Engin, YORUK, Mustafa Deniz, AZKUR, Ahmet Kursat, PESTIL, Zuleyha, and BULUT, Hakan

Subjects

THREE-day sickness in cattle, DISEASE outbreaks, PHYLOGENY, GENES, VETERINARIANS

Abstract

The article focuses on the outbreak of bovine ephemeral fever in Turkey in 2012, including its epidemiology and the molecular characterization of the viruses detected from the outbreak. Topics discussed include the suspected cases reported by Official Veterinarians in many regions in Turkey, and the prevalence of BEFV in the country. Also mentioned is the results of phylogenetic analysis of BEFV isolates based on comparison of G gene sequences.

Published

2013

9. A reverse-transcription PCR method for detecting all known ephemeroviruses in clinical samples.

Author

Blasdell, Kim R., Adams, Mathew M., Davis, Steven S., Walsh, Susan J., Aziz-Boaron, Orly, Klement, Eyal, Tesh, Robert B., and Walker, Peter J.

Subjects

*REVERSE transcriptase polymerase chain reaction, *VIRAL genomes, *VIRUS identification, *VIRUS research, *THREE-day sickness in cattle, *TISSUE culture

Abstract

Highlights: [•] The first single primer pair PCR able to detect all ephemerovirus genus members. [•] This PCR, in conjunction with sequencing, can determine the virus species. [•] This PCR can detect BEFV in both tissue culture isolates and clinical cattle blood. [•] The sensitivity was 500 RNA copies per reaction for BEFV. [•] For KOTV the sensitivity was between 500 and 5000 RNA copies per reaction. [Copyright &y& Elsevier]

Published

2013

10. Phylogenetic relationships of the glycoprotein gene of bovine ephemeral fever virus isolated from mainland China, Taiwan, Japan, Turkey, Israel and Australia.

Author

Fuying Zheng and Changqing Qiu

Subjects

*GLYCOPROTEINS, *THREE-day sickness in cattle, *PHYLOGENY, *CATTLE infections

Abstract

Background: The glycoprotein (G) gene sequences of bovine ephemeral fever virus (BEFV) strains derived from mainland China have not been compared with those of the isolates from other countries or areas. Therefore, the G genes of four BEFV isolates obtained from mainland China were amplified and sequenced. A phylogenetic tree was constructed in order to compare and analyze the genetic relationships of the BEFV isolates derived from mainland China and different countries and areas. Results: The complete BEFV G gene was successfully amplified and sequenced from four isolates that originated from mainland China. A total of fifty-one BEFV strains were analyzed based on the G gene sequence and were found to be highly conserved. A phylogenetic tree showed that the isolates were grouped into three distinct lineages depending on their source of origin. The antigenic sites of G1, G2 and G3 are conserved among the isolates, except for several substitutions in a few strains. Conclusions: The phylogenetic relationships of the BEFV isolates that originated from mainland China, Taiwan, Japan, Turkey, Israel and Australia were closely related to their source of origin, while the antigenic sites G1, G2 and G3 are conserved among the BEFV isolates used in this work. [ABSTRACT FROM AUTHOR]

Published

2012

11. A reverse-transcription, loop-mediated isothermal amplification assay for detection of bovine ephemeral fever virus in the blood of infected cattle

Author

Zheng, Fuying, Lin, Guozhen, Zhou, Jizhang, Wang, Guanghua, Cao, Xiaoan, Gong, Xiaowei, and Qiu, Changqing

Subjects

*REVERSE transcriptase polymerase chain reaction, *PATHOGENIC microorganisms, *DIAGNOSTIC microbiology, *VIRUS diseases in cattle, *GENE amplification, *BIOLOGICAL assay, *THREE-day sickness in cattle, *SENSITIVITY & specificity (Statistics), *VIRUS isolation

Abstract

Abstract: A novel reverse-transcription, loop-mediated isothermal amplification (RT-LAMP) assay for the detection of bovine ephemeral fever virus (BEFV) was developed and evaluated in this study. The RT-LAMP assay exhibited higher sensitivity when compared with conventional reverse-transcription polymerase chain reaction (RT-PCR) and virus isolation methods. The specificity of the assay was determined by digestion of the RT-LAMP products with restriction enzyme and detection of BEFV serogroup rabies virus (RV). Using RT-LAMP, RT-PCR and virus isolation methods, 36 blood samples were tested and the results indicated that RT-LAMP could detect early infection with BEFV. The RT-LAMP method is useful for the diagnosis of BEFV infection in blood samples. [ABSTRACT FROM AUTHOR]

Published

2011

12. Inhibitors of phosphatidylinositol 3-kinase and mTOR but not Akt enhance replication of bovine ephemeral fever virus.

Author

Ji, Wen T., Wang, Ying C., Lin, Feng L., Liao, Ming H., Shih, Wen L., and Liu, Hung J.

Subjects

*RNA viruses, *BOS, *PROTEIN kinases, *THREE-day sickness in cattle, *VIRAL replication, *VETERINARY virology

Abstract

Non-segmented, negative-sense RNA viruses (NNSVs) depend on Akt (protein kinase B) for efficient replication. Infection with bovine ephemeral fever virus (BEFV) increases Akt phosphorylation. This study examined the effect of inhibition of phosphatidylinositol 3-kinase (PI3K)-Akt signalling on BEFV replication, since PI3K is the major upstream regulator of Akt. Treatment of BEFV-infected cells with two specific PI3K inhibitors (wortmannin and LY294002) enhanced replication of BEFV when compared to the effects of Akt inhibitors Ill and IV. BEFV antagonised the effects of PI3K inhibitors on Akt dephosphorylation. Inhibition of roTOR by rapamycin also enhanced replication of BEFV. The results provide evidences that inhibition of PI3K and mTOR has positive effects on replication of BEFV. [ABSTRACT FROM AUTHOR]

Published

2011

13. Serological detection of bovine ephemeral fever virus using an indirect ELISA based on antigenic site G1 expressed in Pichia pastoris.

Author

Fu-Ying Zheng, Guo-Zhen Lin, Chang-Qing Qiu, Ji-Zhang Zhou, Xiao-An Cao, and Xiao-Wei Gong

Subjects

*SERODIAGNOSIS, *THREE-day sickness in cattle, *PICHIA pastoris, *ANTIGENS, *IMMUNOGLOBULINS

Abstract

An indirect ELISA for the serological detection of bovine ephemeral fever virus (BEFV) infection in cattle is described in which a glycosylated protein of approximately 25 kDa (including the G1 antigenic site of the virus glycoprotein) expressed in Pichia pastoris GSI 15 was used as the coating antigen. The optimal concentration of coated antigen was 0.3 µg/well at a serum dilution of 1:40. The optimal positive threshold value of the assay was 1.88, as derived from receiver operating characteristic curve analysis. The test had 100% sensitivity and 96.7% specificity when compared with a micro-neutralisation test using 336 positive and 180 negative sera to BEFV, respectively. The inter-assay and intra-assay coefficients of variation for 15 sera were both <5.8% and there was no evidence of cross-reactivity between the tested coating antigen and antibodies to related rabies virus. The ELISA is an inexpensive and rapid serological detection method that would be suitable for screening for BEFV infection on a large scale. [ABSTRACT FROM AUTHOR]

Published

2010

14. Phylogenetic relationships of the G gene sequence of bovine ephemeral fever virus isolated in Japan, Taiwan and Australia

Author

Kato, Tomoko, Aizawa, Maki, Takayoshi, Katsunori, Kokuba, Tamotsu, Yanase, Tohru, Shirafuji, Hiroaki, Tsuda, Tomoyuki, and Yamakawa, Makoto

Subjects

*NUCLEOTIDE sequence, *THREE-day sickness in cattle, *ANIMAL health, *PHYLOGENY, *VIRUS isolation, *MOLECULAR epidemiology, *VETERINARY epidemiology, *MEDICAL genetics

Abstract

Abstract: The G gene encoding the neutralization antigen of bovine ephemeral fever virus (BEFV) was characterized in order to define the virus''s molecular epidemiology in Japan and the genetic relationships among the Japanese, Taiwanese and Australian isolates. The nucleotide and amino acid sequences of the gene were highly conserved among the Japanese strains, regardless of the year of isolation, and were closely related to the Taiwanese strains. By phylogenetic analysis, the Japanese and Taiwanese strains were classified clearly into three chronological clusters: 1966, 1984–1989 and 1996–2004, indicating that the epidemics of bovine ephemeral fever may occur almost simultaneously in both countries by the same genotype. On the other hand, the Australian strains were distantly related to these East Asian strains and placed in the independent fourth cluster of the phylogenetic tree. It is suggested that three amino acid substitutions at residues 224, 271 and 499 in the neutralizing epitopes, of which two generate new glycosylation sequences, are responsible for antigenic variations of bovine ephemeral fever virus. The cross-neutralization test using the bovine ephemeral fever virus isolated in Japan demonstrated that the vaccine developed based on the oldest Japanese strain, YHL, appears to still be effective for controlling bovine ephemeral fever in Japan. [Copyright &y& Elsevier]

Published

2009

15. Development of a reliable assay protocol for identification of diseases (RAPID)-bioactive amplification with probing (BAP) for detection of bovine ephemeral fever virus

Author

Hsieh, Yao-Ching, Chen, Shih-Hui, Chou, Chin-Sheng, Hsiao, Hsu-Wen, Chen, Shu-Zhen, Lee, Yen-Feng, and Liu, Hung-Jen

Subjects

*THREE-day sickness in cattle, *CATTLE infections, *DENGUE, *VIRUSES

Abstract

Abstract: A rapid, sensitive, and specific assay, RAPID-BAP assay, was developed to detect and quantify the G protein-encoding gene of bovine ephemeral fever virus (BEFV). This new technique uses a nested PCR and magnetic bead-based DNA probing assay. The optimal conditions for the assay were examined. By applying a nested PCR, a minimum of 1 copy/μl of the BEFV plasmid DNA could be detected by the assay. The optimal hybridization conditions at 50°C in 5× SSC and 0.5% SDS with a 20-min incubation allowed clear discrimination between negative and positive controls. The assay was also highly specific as all negative controls failed to show any positive detection. The diagnostic sensitivity of the RAPID-BAP assay, real-time RT-PCR, and conventional RT-PCR in the detection of 34 clinical blood samples suspected to have BEFV infections were 72.73, 36.36, and 18.18%, respectively. The results indicated that the RAPID-BAP assay developed in this study was more sensitive than the conventional RT-PCR and real-time RT-PCR assays for the detection of BEFV. The novel RAPID-BAP assay is an excellent diagnostic tool with high sensitivity, specificity, and fast turnaround time. [Copyright &y& Elsevier]

Published

2005

16. Determination of the oral susceptibility of South African livestock-associated biting midges, Culicoides species, to bovine ephemeral fever virus.

Author

Venter, G. J., Hamblin, C., and Paweska, J. T.

Subjects

*CULICOIDES, *LIVESTOCK, *THREE-day sickness in cattle

Abstract

Abstract. A total of 10 607 Culicoides midges (Diptera: Ceratopogonidae) were fed on either sheep or horse blood containing not less than 6.5 log10 TCID50 /ml of bovine ephemeral fever virus (BEFV). Insects were collected during two consecutive summers from two distinct climatic areas. Two seed viruses, originating from either South Africa or Australia, were used separately in the feeding trials. Blood-engorged females were incubated at 23.5°C for 10 days and then individually assayed in microplate BHK-21 cell cultures. Of the 4110 Culicoides that survived, 43% were C. (Avaritia ) imicola Kieffer and 27% were C. (A. ) bolitinos Meiswinkel. The remainder represented 18 other livestock-associated Culicoides species. Although BEFV was detected in 18.9% of midges assayed immediately after feeding, no virus could be detected after incubation. The absence of evidence of either virus maintenance or measurable replication suggests that most of the abundant livestock-associated Culicoides species found in South Africa are refractory to oral infection with BEFV. Future studies should be carried out using species of mosquitoes that are associated with cattle in the BEF endemic areas. [ABSTRACT FROM AUTHOR]

Published

2003

17. Development and application of G1-ELISA for detection of antibodies against bovine ephemeral fever virus

Author

Zheng, Fu-ying, Lin, Guo-zhen, Qiu, Chang-qing, Zhou, Ji-zhang, Cao, Xiao-an, and Gong, Xiao-wei

Subjects

*ENZYME-linked immunosorbent assay, *VIRAL antibodies, *THREE-day sickness in cattle, *GENETIC code, *BACTERIAL genetics, *ESCHERICHIA coli, *HOST-virus relationships, *RECOMBINANT proteins, *MICROBIAL sensitivity tests

Abstract

Abstract: The gene encoding antigenic site G1 of bovine ephemeral fever virus (BEFV) was highly expressed in the host cell Escherichia coli. An indirect G1-ELISA with the recombinant protein as the coating antigen was established to detect antibodies against BEFV. The result revealed that the optimal concentration of the coated antigen was 0.5μg/well and the dilution of serum was 1:20. It was optimal that sera with P/N value⩾2.2 were considered positive, P/N value⩽2.0 negative, and between 2.0 and 2.2 ambiguous. The G1-ELISA method gave a sensitivity of 97.6% and a specificity of 98.6% by testing 590 field serum samples. These results suggest that the G1-ELISA may be a good alternative tool for seroepidemiological surveys. [Copyright &y& Elsevier]

Published

2009