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11.
Grouper Epinephelus spp. is one of the most important mariculture fish species in China and South-East Asian countries. The emerging viral diseases, evoked by iridovirus which belongs to genus Megalocytivirus and Ranavirus, have been well characterized in recent years. To date, few data on lymphocystis disease in grouper which caused by lymphocystis disease virus (LCDV) were described. Here, a novel LCDV isolate was identified and characterized. Based on the sequence of LCDV major capsid protein (MCP) and DNA polymerase gene, we found that the causative agents from different species of diseased groupers were the same one and herein were uniformly defined as grouper LCDV (GLCDV). Furthermore, H&E staining revealed that the nodules on the skin were composed of giant cells that contained inclusion bodies in the cytoplasm. Numerous virus particles with >210 nm in diameter and with hexagonal profiles were observed in the cytoplasm. In addition, phylogenetic analysis based on four iridovirus core genes, MCP, DNA polymerase, myristoylated membrane protein (MMP) and ribonucleotide reductase (RNR), consistently showed that GLCDV was mostly related to LCDV-C, followed by LCDV-1. Taken together, our data firstly provided the molecular evidence that GLCDV was a novel emerging iridovirus pathogen in grouper culture. 相似文献
12.
大鲵虹彩病毒流行株的分离及其主衣壳蛋白编码基因序列比较分析 总被引:1,自引:1,他引:0
大鲵虹彩病毒(giant salamander iridovirus, GSIV)是近年中国大陆新发现的引起人工养殖大鲵(Andrias davidianus)大规模死亡的病毒病原。为了揭示大鲵虹彩病毒流行株的基因型差异, 本研究对2010–2012年采集自全国不同大鲵养殖区域的患虹彩病毒病的大鲵样本进行了分子检测、病毒分离培养以及病毒主衣壳蛋白(major capsid protein, MCP)基因测序与比对分析。结果显示, 采自陕西、湖北、湖南、浙江、江西、福建等省的10个样本检测为阳性, 通过细胞培养获得10株病毒流行株。对该10株流行株MCP基因的测序与比对分析发现, 核苷酸序列相似性达到99.7%~100%, 其推测的氨基酸序列无明显差异, 证实中国大鲵虹彩病毒流行株属同一基因型。系统进化树分析结果表明, 所选大鲵虹彩病毒与蛙病毒分别聚为一枝, 但其亲缘关系较近。本研究结果旨为大鲵虹彩病毒病的疫苗研制及其免疫防控技术研究奠定基础。
相似文献13.
2013年7月,陕西省汉中某大鲵养殖场发生以大鲵体表和四肢多处溃烂并伴有出血为特征的疾病,染病大鲵大量死亡。经临床观察、病理解剖及实验室检测,最后确诊病原为大鲵虹彩病毒。通过采取综合防治措施,养殖场大鲵疫情得到有效控制。 相似文献
14.
大鲵虹彩病毒TaqMan实时荧光定量PCR检测方法的建立 总被引:4,自引:2,他引:2
利用PCR技术扩增出大鲵虹彩病毒(giant salamander iridovirus, GSIV)主要衣壳蛋白(MCP)编码区长度为1 392 bp 的片段, 克隆到 pMD19-T载体上, 构建重组质粒 pMD19-T-MCP。经PCR鉴定确认正确后, 以10倍梯度稀释 pMD19-T-MCP重组质粒, 作为标准模板进行 TaqMan实时荧光定量PCR扩增, 制作标准曲线, 建立了大鲵虹彩病毒的 TaqMan实时荧光定量PCR检测方法。制作的标准曲线有极好的线性关系, 且线性范围宽, 相关系数为0.990 19。组内重复试验的CT值标准偏差为0.52%。检测结果显示, 该方法对大鲵虹彩病毒的检测有高度的特异性, 与锦鲤疱疹病毒、弗氏柠檬酸杆菌、嗜水气单胞菌以及鲤上皮瘤细胞基因组DNA之间均无交叉反应, 特异性好, 检测总DNA灵敏度为10个病毒核酸分子拷贝数, 约1.1×10-3 pg/μL病毒核酸, 较之常规PCR的敏感度高出约1 000倍。研究建立的大鲵虹彩病毒TaqMan实时荧光定量PCR方法灵敏度高、特异性强, 对大鲵虹彩病毒病的快速诊断与病毒病原定量检测有重要意义。 相似文献
15.
大鲵虹彩病毒理化及生物学特性研究 总被引:8,自引:1,他引:7
对大鲵虹彩病毒(Giant salamander iridovirus,GSIV)的理化特性及生物学特性进行了研究。结果表明:GSIV对热处理敏感,56℃和65℃处理30 min均可彻底灭活病毒;GSIV经酸(pH3)和碱(pH10)处理,病毒滴度(TCID50)与对照组相比较分别下降了8.58、9.04个对数级,差异极显著(P<0.01);GSIV经有机溶剂氯仿、乙醚以及胰蛋白酶处理,TCID50与对照组相比较分别下降了9.33、7.83、6.49个对数级,差异极显著(P<0.01)。冻融次数对GSIV滴度的影响不显著(P>0.05)。GSIV对细胞培养物的感染性试验结果表明,GSIV可在鲤上皮瘤细胞系(Epithelioma papilloma cyprini,EPC)、斑点叉尾鮰肾脏细胞系(Channel catfish kidney,CCK)、虹鳟鱼性腺细胞系(Rainbow trout gonadal,RTG-2)等细胞中增殖,但在EPC、CCK细胞中增殖速度快,TCID50高;GSIV在EPC细胞中的最适生长温度是25℃。GSIV在EPC细胞中增殖动态试验结果表明,GSIV感染细胞6 h后TCID50开始快速上升,进入对数增长期,72 h时TCID50达到最大值,以后趋于稳定。GSIV感染EPC细胞超薄切片透射电镜观察结果显示,在EPC细胞质中可见大量虹彩病毒样颗粒,呈晶格状排列,直径约140 nm。 相似文献
16.
Approximately 8 weeks after a chlorine insult associated with the city water supply, shortnose sturgeon, Acipenser brevirostrum (L.), from one group presented with small (3–4 mm) irregular foci of cutaneous pallor that involved the dorsocranial integument with progressive ulceration of the nascent lesions. Various bacterial organisms were isolated from the cutaneous lesions, but not from the internal viscera. Histologically, the nuclei of the intralesional and perilesional epidermal cells often exhibited margination of the chromatin that resulted in a homogenous, pale, amphophilic, tinctorial quality of the nucleoplasm consistent with a herpesvirus infection. In addition, rare lamellar epithelial cells were prominently enlarged due to an abundant, dense, basophilic cytoplasm characteristic of an iridovirus infection. Inoculation of cutaneous lesion and kidney, spleen, liver sample pools from affected shortnose sturgeon onto white sturgeon spleen (WSS‐2) cell line induced cytopathic effect characterized by syncytia formation. Ultrastructural analysis of infected WSS‐2 cells revealed viral particles with a characteristic herpesvirus morphology. Intranuclear hexagonal capsids had a diameter of 95–108 nm, and enveloped particles present in the cytoplasm of infected cells had a diameter of 176–196 nm. This is the first report of a herpesvirus and a possible iridovirus‐like infection in shortnose sturgeon. 相似文献
17.
根据大鲵虹彩病毒(Chinese giant salamander iridovirus,GSIV)主要衣壳蛋白(Major Capsid Protein,MCP)基因设计引物,PCR扩增得到MCP基因编码框全长序列1 392 bp,将其克隆到原核表达载体p ET-32a中,构建了重组原核表达载体p ET-32a-MCP,并在大肠杆菌BL21中得到了表达,融合表达的重组蛋白分子量约为70 ku,与预期大小一致,主要以包涵体的形式存在。对IPTG浓度,诱导温度等诱导表达条件进行优化,确定0.5 mmol/L的IPTG于37℃的条件下诱导6 h重组蛋白的表达量最佳。纯化GSIVMCP重组蛋白免疫新西兰大白兔,制备了GSIV-MCP多克隆抗体,ELISA检测抗体效价大于1∶50 000。Western blot检测显示该抗体可以特异性识别重组蛋白。间接荧光免疫结果表明,该多克隆抗体可与由GSIV感染引起细胞病变的EPC细胞(GICB)发生特异性的结合。研究为建立GSIV免疫诊断方法以及为研究GSIV MCP基因编码蛋白的功能奠定了前期基础。 相似文献
18.
【目的】花鲈虹彩病毒(Lateolabrax maculatus iridovirus,LMIV)严重威胁花鲈养殖业安全,无特效防控药物,早期诊断在LMIV防控中发挥极其重要的作用。建立一种简便、快捷、准确的现场快速诊断方法,可为LMIV的基层诊断提供技术支撑。【方法】利用交叉引物恒温扩增技术(Cross priming amplification,CPA),针对LMIV ATPase基因高保守区设计1套单交叉引物。以构建的ATPase重组质粒作为阳性模板,对反应体系中的引物浓度比,Bst DNA聚合酶、Betaine、MgSO4、dNTP浓度,以及反应温度和反应时间进行优化;结合一次性核酸试纸条,建立可视化检测LMIV-CPA的方法。【结果】最优引物浓度比组合为交叉引物CPF1.0μmol/L,引物F3和B3均为0.4μmol/L,探针引物B1(FAM)和B2(Biotin)均为0.8μmol/L;MgSO4浓度为6 mmol/L、Betaine浓度为0.4 mol/L、dNTP浓度为0.6 mmol/L、Bst DNA聚合酶浓度为0.256 U/μL;最佳反应... 相似文献
19.
Pallister J Gould A Harrison D Hyatt A Jancovich J Heine H 《Journal of fish diseases》2007,30(7):427-438
Serious systemic disease in fish and amphibians is associated with the ranaviruses, epizootic haematopoietic necrosis virus (EHNV) and Bohle iridovirus (BIV) in Australia, and European sheatfish virus (ESV) and European catfish virus (ECV) in Europe. EHNV, ESV and ECV are recognized causative agents of the OIE (Office International des Epizooties) notifiable systemic necrotizing iridovirus syndrome and are currently identified by protein-based assays, none of which are able to rapidly identify the specific agents. The aim of this study was to develop TaqMan real-time PCR assays that differentiated these viruses using nucleotide sequence variation in two ranavirus genes. A conserved probe representing 100% sequence homology was used as a reference for virus-specific probes. The virus-specific probes produced a similar signal level to the conserved probe while those probes binding to non-target viral DNA produced an altered fluorescent curve. The pattern of probe binding was characteristic for each virus. Sensitivity, specificity and dynamic range of the assay were assessed. The test is currently useful as a research and initial screening tool, with the potential to become a sensitive and specific method for detection and differentiation of ranaviruses with further development. 相似文献
20.
Drennan JD Lapatra SE Samson CA Ireland S Eversman KF Cain KD 《Journal of fish diseases》2007,30(6):367-379
Pectoral fin tissue of white sturgeon was investigated as a potential non-lethal sample source for the detection of white sturgeon iridovirus (WSIV) infection. Histopathology and polymerase chain reaction (PCR) results using fin tissue were compared with the standard lethal histopathology sampling method that utilizes head tissue. Tissues for each of the three sampling methods were collected weekly for 8 weeks from individual sturgeon undergoing an experimental cohabitation challenge with fish infected with the Abernathy isolate of WSIV. Non-lethal fin histopathological evaluation did not reveal infection during the first 3 weeks of sampling, while non-lethal PCR and the lethal method were variable. However, all three sampling methods were equally capable of identifying infection from 4 to 8 weeks post-exposure. Of the survivors tested, all were negative by PCR and the lethal method, and only one fish was identified as being positive by non-lethal fin histopathology. In another experiment, all three sampling methods were applied to asymptomatic WSIV carriers in a case study conducted at the Kootenai Tribal Sturgeon Conservation Hatchery. Results showed that both lethal and non-lethal fin histopathology were equally effective in detecting infection, but PCR was unable to identify this strain of WSIV. Depending on the virus isolate, these results suggest that non-lethal sampling of fin tissue (histopathology or PCR) is comparable with the lethal sampling method at identifying WSIV infection once infection is established, and under certain circumstances may provide an alternative to lethal sampling. 相似文献