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1.
J H Park H Kida K Ueda K Ochiai M Goryo C Itakura 《Zentralblatt für Veterin?rmedizin. Reihe B. Journal of veterinary medicine. Series B》1991,38(10):749-754
Causative agent of rabbit haemorrhagic disease (RHD) was purified by CsCl density gradient centrifugation from the liver homogenate of rabbits infected with RHD virus which originated from Korea. The viral particles were 35-40 nm in diameter, and had hollow depressions on their surface. Protein A-gold immunoelectron microscopy clearly showed that the convalescent antisera of diseased rabbits reacted specifically with the virus particles. SDS-PAGE and Western blot analyses demonstrated that the structural protein of the virus was composed of a single major polypeptide of 63 kD. These findings indicate that the causative agent of RHD, tentatively named as picornavirus in Korea, belongs to calicivirus. 相似文献
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R C Povey 《American journal of veterinary research》1978,39(1):175-178
Ribavirin had marked in vitro activity against feline calcivirus, strain 255, and canine parainfluenza virus, but showed only slight antiviral effect on feline viral rhinotracheitis virus. Antiviral activity was manifested by partial to complete suppression of viral cytopathic effect and of viral replication, depending on concentration of ribavirin in the culture medium and dosage of viral inoculum. Concentrations of ribavirin as small as 3.2 microgram/ml and 1.0 microgram/ml showed some activity against feline calcivirus and canine parainfluenza virus, respectively. 相似文献
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Characterization of swine infertility and respiratory syndrome (SIRS) virus (isolate ATCC VR-2332). 总被引:35,自引:0,他引:35
D A Benfield E Nelson J E Collins L Harris S M Goyal D Robison W T Christianson R B Morrison D Gorcyca D Chladek 《Journal of veterinary diagnostic investigation》1992,4(2):127-133
The characterization of an isolate of swine infertility and respiratory syndrome (SIRS) virus (ATCC VR-2332) is reported. A commercial cell line (CL2621) was used for the propagation of the virus for all assays. Laboratory studies indicate that this isolate is a fastidious, nonhemagglutinating, enveloped RNA virus. Cesium chloride-purified virions visualized by electron microscopy were spherical particles with an average diameter of 62 nm (range: 48-83 nm) and a 25-30 nm core surrounded by an envelope. Virus replication was restricted to the cytoplasm, as demonstrated by immunofluorescence. The virus did not react serologically with antisera to several common porcine viruses or with antisera to known viruses in the alphavirus, rubivirus, pestivirus, and ungrouped lactic dehydrogenase virus genera of the Togaviridae. However, convalescent sow sera and rabbit hyperimmune sera neutralized the SIRS virus at titers of 1:256 and 1:512, respectively. The virus was stable at 4 and -70 C, but was labile at 37 and 56 C. The properties of this isolate of SIRS virus resemble those of the family Togaviridae but do not match the described genera. 相似文献
4.
Siri Vike Karin Oelckers Henrik Duesund Svein Rune Erga Javier Gonzalez Børge Hamre 《Journal of aquatic animal health》2013,25(1):33-42
AbstractInfectious salmon anemia (ISA) virus (genus Isavirus, family Orthomyxoviridae), present in all major salmon producing countries, is the causative agent for a serious and commercially important disease affecting Atlantic Salmon Salmo salar. Nearly all ISA outbreaks occur in the marine production phase and knowledge about survival time for ISA virions in seawater is crucial for an adequate strategy to combat the disease. To acquire knowledge about this important factor, a study of ISA virus exposed to four different physical conditions was carried out. The virions’ survival was tested in sterile seawater, sterile seawater with normal ultraviolet light radiation (UVR), natural seawater, and natural seawater with UVR. During the 72-h experiment both presence of ISA virus RNA and the infectivity of ISA virions were monitored. The result of this study showed that the infectivity of ISA virions is lost within 3 h of exposure to natural seawater or sterile seawater with UVR. However, it was possible to detect ISA virus RNA throughout the experimental period. This indicates that the effect of both UVR and biological activity of natural seawater limits the survival time of ISA virions under normal conditions. The survival time of ISA virions in sterile seawater was less than 24 h. Based on the available literature and the present study it is not very likely that passive horizontal transmission in seawater over long distances can occur. This is due to the following factors: (1) the effect of UVR and biological activity on ISA virions infectivity found in the present study, (2) the speed and dilution effect in seawater currents in salmon farming areas, (3) the temperature during the major outbreak periods, and (4) the need for an infective dose of ISA virions to reach naive Atlantic Salmon.Received August 22, 2013; accepted November 7, 2013 相似文献
5.
以建立的斑点酶联免疫吸附试验双抗体夹心法检测兔出血症病毒抗原.结果表明,对23只病兔各脏器病毒抗原检测,以肝、脾的检出率为最高.对人工感染兔各脏器检测,肝脏首先出现病毒抗原,其次是脾脏;各脏器病毒抗原含量依次为,肝>脾>肺>肾>心.用该法从人工感染24h后兔的口腔、鼻腔分泌物及粪便中检出了病毒抗原,表明病兔可通过消化道和呼吸道排毒.与血凝试验对比检测兔出血症可疑标本192份,两者符合率为90.6%. 相似文献
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Porcine reproductive and respiratory syndrome virus: morphological, biochemical and serological characteristics of Quebec isolates associated with acute and chronic outbreaks of porcine reproductive and respiratory syndrome. 总被引:7,自引:2,他引:5 
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下载免费PDF全文 Cytolytic and noncytolytic strains of the porcine reproductive and respiratory syndrome virus (PRRSV) were isolated in primary cultures of porcine alveolar macrophages (PAM) from lung homogenates of stillborn fetuses or blood samples of dyspneic piglets collected from Quebec pig farms having experienced acute or chronic outbreaks of PRRS. Serological identification of the virus was confirmed by indirect immunofluorescence and indirect protein A-gold immunoelectron microscopy using reference antiserum prepared from experimentally-infected specific pathogen free (SPF) piglets and monoclonal antibodies (MoAbs) directed against the p15 nucleocapsid (N) protein of the reference ATCC-VR2332 isolate. Intracytoplasmic enveloped viral particles that tended to accumulate into cytoplasmic vesicles were observed in the infected PAM; no budding was demonstrated at the level of the cytoplasmic membrane. The extracellular virions appeared as pleomorphic but mostly spherical enveloped particles, 50-72 nm in diameter (averaged diameter of 50 particles was 58.3 nm), with an isometric core about 25-30 nm. Buoyant density of the virus in CsCL density gradients was estimated to 1.18-1.20 g/mL. No hemagglutinating activity was demonstrated. Analysis of semipurified virions of isolate IAF-exp91 by radioimmunoprecipitation (RIPA) and Western immunoblotting experiments, using reference rabbit and porcine hyperimmune sera, revealed four major viral proteins, a predominant 15 kD N protein and three other proteins with predicted M(r_ of 19, 26 and 42 kD. Progeny viral particles produced in PRRSV-infected PAM in the presence of tunicamycin lacked the 42 kD protein, thus confirming its N-glycosylated nature. Immunoprecipitation experiments using the anti-ATCC-VR2332 MoAbs confirmed the close antigenic relationships between Quebec and American reference isolates of PRRSV. 相似文献
7.
兔出血症病毒在细胞培养和组织中的形态发生 总被引:4,自引:2,他引:2
在电镜下系统地观察了感染后的细胞培养和组织中兔出血症病毒( R H D V)的形态发生。感染早期,在细胞核内可见电子致密颗粒(15 nm )和未成熟的病毒颗粒 (25 nm )。中期,在细胞核和胞浆内出现大量成熟的病毒颗粒(34 nm ),并发现部分核内病毒通过扩大的核膜孔、核膜溶解扩大的核孔和乳头状突起的核膜向胞浆释放。感染末期,核染色质消失,核内大量感染病毒清淅可见。最终细胞溶解,病毒颗粒释放至细胞间隙。提示 R H D V 是在核内复制和装配的,应归属于细小病毒科。本试验结果不排除同时存在另一种小 R N A 病毒。 相似文献
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H J Cho 《Canadian journal of veterinary research》1977,41(2):215-218
A highly purified and concentrated suspension of aleutian disease virus was prepared from large quantities of early infected mink tissues using repeated fluorocarbon extraction procedures. Equilibrium centrifugation of the aleutian disease virus preparation in a cesium chloride gradient yielded three distinct bands at buoyant densities of 1.295, 1.332, and 1.405--1.416 g/cm(3). Electron microscopic observations of these three bands revealed mainly empty particles in the first band. In the second band complete particles with a flattened appearnce predominated and there were also some empty particles. In the third band both complete and empty particles were observed. The size of the aleutian disease virus particles observed in all of the three densities was 23 nm. Light aleutian disease virions (density of 1.332 g/cm3) had a particle to counterimmunoelectrophoresis antigen ratio comparable to that of dense aleutian disease virions (density of 1.405--1.416 g/cm3) but possessed much lower infectivity as determined by mink inoculation. 相似文献
10.
The present paper refers to the cytometric analysis of lymphocytes T (with receptor CD5+), Th (with receptor CD4+), Tc/Ts (with receptor CD8+), lymphocytes CD25+ and lymphocytes B with receptor CD19+ in rabbits experimentally infected with strains of RHD virus--Rainham, Frankfurt and Asturias, not having haemagglutinogenic capacities, which makes them unique, as haemagglutinogenic capacity is a classic and typical property of most strains of this virus. The study was performed in the dynamic system, drawing blood samples from animals at hour 0, namely before the administration of the viral antigen, and then at 4, 8, 12, 24 and 36 h after the infection. The study indicated that Rainham and Asturias strains of RHD virus cause a similar amount of changes as the most immunogenic haemagglutinogenic strains CAMP V-561 and CAMP V-562 of the RHD virus do. In contrast, the Frankfurt strain of the RHD virus is characterised with 5-6-fold lower reactivity in this respect and is most similar to the least immunogenic haemagglutinogenic strain CAMP V-558 of the RHD virus. 相似文献
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兔病毒性出血症基因工程苗研究概况 总被引:5,自引:0,他引:5
由于兔病毒性出血症 (RHD)组织灭活苗涉及的成本、生物安全及动物福利等问题 ,国内外学者正致力于 RHD新型疫苗的研制和开发。以 VP60表达为基础的亚单位疫苗经历了最初的原核、真核表达 ,目前正寻求在转基因植物中进行表达 ,以期获得大量、低成本的口服疫苗 ;而以牛痘、金丝雀痘病毒、黏液瘤病毒等作载体的重组活载体苗 ,无疑使 RHD疫苗正在向更安全、实用及对家兔、野兔均有保护作用方向发展 ,具有很大的发展潜力和前景。国外学者在RHD基因工程苗方面研究较为广泛和深入 ,而国内尚未有此方面报道 相似文献
13.
Identification of envelope and nucleocapsid proteins of infectious bovine rhinotracheitis virus by SDS-polyacrylamide gel electrophoresis 总被引:9,自引:0,他引:9
Infectious bovine rhinotracheitis (IBR) virus was purified by rate zonal and isopycnic centrifugation in potassium tartrate gradients. Viral nucleocapsids were isolated from purified virions by treatment with the nonionic detergent Triton X-100 followed by high speed centrifugation. This treatment was shown to produce a suspension of 74% completely de-enveloped nucleocapsids, 24% incompletely de-enveloped nucleocapsids, and 2% whole virions. The viral nucleocapsids contained DNA and banded at a density of 1.25 g/cm3. Analysis of the viral polypeptides by gradient SDS-polyacrylamide gel electrophoresis revealed that 33 virion proteins, ranging in molecular weight from 13,000 to 275,000 dalton, were present in the complete virus particle. Detergent treatment of the virus quantitatively removed two of the major proteins (vp8, 90,000 dalton, and vp13, 73,000 dalton) and partially removed eleven other proteins. Fifteen viral polypeptides appeared to remain firmly associated with the viral nucleocapsids. 相似文献
14.
M Hessami D A Keney L D Pearson J Storz 《Comparative immunology, microbiology and infectious diseases》1979,2(1):1-7
Maculopapular, pock-like lesions were detected repeatedly on hands and arms of students having contact with sheep or cattle. Pustular lesions were seen on the mammary gland and vulva of a goat. Biopsy samples of the lesions from 3 students and the goat were cultured on bovine fetal spleen (BFS) cells. Viruses were isolated from all samples. The viral isolates induced similar cytopathic changes in BFS cells. Slowly spreading plaque-like changes consisting of large, round cells developed in BFS monolayers. In a growth curve experiment involving the Shoe strain and BFS cells, virus infectivity increased 8 hr after inoculation. The major portion of the infectivity remained associated with the cell fraction. Maximal titers were found 36 hr after infection. Eosinophilic inclusions of varying size were detected in the cytoplasm 8–18 hr after infection of BFS cells. Later these inclusions enlarged, coalesced, stained basophilically, and remained attached to the pycnotic nuclei. Vacuoles created a ballooning appearance and separated the plasma membrane from the nucleus-viral inclusion complex by 24 hr after infection when the cells detached. Negatively stained preparations of purified virus of the isolates contained ovoid virions covered with diagonally woven bands. The long axis of the virions measured 220 and 250 nm and the short axis was 120–140 nm. These features are characteristic of the parapox virus genus which includes members that induce orf. 相似文献
15.
D Fargeaud M Bugand P Précausta J P Soulebot J Tektoff 《Comparative immunology, microbiology and infectious diseases》1982,5(1-3):39-47
The thermal degradation of rabies virus was determined by the variation in optical density at 260 nm during temperature rise. This variation, linked to denaturation of RNA, was seen by an irreversible sigmoidal curve. Analysis of the state of the virion by ultracentrifugation did not show any alteration in sedimentation. Electron microscopy revealed a release of nucleic acid of the virions which were burst to a greater or lesser degree. The technical conditions of these measurements--speed of temperature rise and virus preparation--are defined. The form of the curve and the different measurements which develop from it, enable the influence of numerous factors linked either to the sodium, calcium and magnesium environment, or to an alteration of the virus by chemical substances, especially inactivation agents, to be observed. The study of the thermal degradation of rabies virus is an interesting method of determining the action of different factors on the stability of the virion. 相似文献
16.
H Liebermann H Bergmann E Lange H Schirrmeier P Solisch 《Zentralblatt für Veterin?rmedizin. Reihe B. Journal of veterinary medicine. Series B》1992,39(5):317-326
Purified and concentrated preparations of virus from liver extracts of infected rabbits contain virus specific components with sedimentation coefficients of about 175, 110 and sometimes 133S and more slow units. Full and empty virus particles with a diameter of about 34 nm were shown electron microscopically in the corresponding 175 and 110S fractions of the sucrose density gradient. The average of buoyant density of the 175, 133, 110S and more slow units are 1.36, 1.32 and 1.31 g/ml respectively. The extinction coefficient E260 nm is 4.3 +/- 0.7 cm2/mg. The RNA content is 17 +/- 4%. SDS-PAGE shows a "65" kD protein as a single or major component. Beside smaller polypeptides with lower intensities, the 67 kD polypeptide reacts positively in the Western blot with polyclonal antibodies of rabbits. The molecular weight of the virus is 15 +/- 4 x 10(6)D. The pH stability of the 175S unit was also tested. 相似文献
17.
Marchandeau S Bertagnoli S Peralta B Boucraut-Baralon C Letty J Reitz F 《The Veterinary record》2004,155(19):589-592
Serological data on myxoma virus, rabbit haemorrhagic disease (RHD) virus and RHD-like viruses in juvenile rabbits (Oryctolagus cuniculus) trapped in 1995, 1996 and 1997 in two areas of France were analysed. For each disease, the effects of bodyweight, year, month and seropositivity for the other disease were modelled by using logistic regressions. In one area, a model including RHD seropositivity was selected to explain the myxoma virus seropositivity. Models including myxoma virus seropositivity were selected to explain the RHD seropositivity in both areas, and the odds of a rabbit being seropositive to both viruses were 5.1 and 8.4 times higher than the odds of a rabbit being seronegative to myxoma virus and seropositive to RHD. The year and bodyweight had significant effects for myxomatosis in one area and for RHD in both areas. 相似文献
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Fowlpox virus (FWPV), an important pathogen of poultry, replicates very efficiently in the featherless areas of skin, and persists in dried and desiccated scabs for prolonged periods. Although the molecular mechanisms underlying the stability of the virus are not completely known, we recently identified the presence of a virus-encoded novel DNA repair enzyme, CPD-photolyase, in FWPV. This enzyme repairs the ultraviolet (UV)-induced pyrimidine dimers, converting them to monomers using photons from white light as a renewable source of energy. In this study, we examined the role of photolyase in the pathogenesis of fowlpox. A comparison of pathogenesis of fowlpox in chickens infected with parental FWPV with that in chickens infected with photolyase-deficient FWPV (Phr(-) FWPV) found no significant differences in terms of replication of virus or formation of secondary lesions. When the virions isolated from infected scabs were exposed to UV light, UV-damaged parental FWPV, unlike Phr(-) FWPV, were rescued through the CPD-photolyase-mediated photoreactivation pathway by at least 48%. However, the mutant virus triggered host's immune response and conferred complete protection against subsequent challenge with virus similar to that conferred by the parental virus. Since the mutant virus is less stable than the parental virus in the infected scabs but is as immunogenic, Phr(-) FWPV might be less persistent in the environment. Furthermore, this particular genetic locus can also be used to insert foreign genes for the development of FWPV recombinant vaccines. 相似文献
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Peste des petits ruminants virus (PPRV) has a non-segmented negative sense RNA genome and is classified within the Morbillivirus genus of the Paramyxoviridae. Using the Bac-to-Bac® baculovirus expression system, we constructed recombinant baculoviruses that were able to co-express the PPRV matrix and nucleocapsid proteins in insect cells under the control of the polyhedron and p10 promoters, respectively. The results showed that although both structural proteins were expressed at a relatively low level, the interaction between them caused the formation of virus-like particles (VLPs) by viewing of transmission electron microscopy. The VLPs morphologically resembled authentic PPRVs but lacked spikes protruding from the particulate surfaces. Interestingly, the diameter of PPRV VLPs ranged from 100 to 150 nm, far less than the mean diameter (400–500 nm) of parental virions. 相似文献