鸭瘟病毒的分离与初步鉴定

程晓霞; 林锋强; 黄梅清; 肖世峰; 江斌; 吴南洋; 陈少莺; 俞伏松

doi:10.19303/j.issn.1008-0384.2017.08.005

鸭瘟病毒的分离与初步鉴定

doi: 10.19303/j.issn.1008-0384.2017.08.005

程晓霞^{1, 2},
林锋强^{1, 2},
黄梅清^{1, 2},
肖世峰^{1, 2},
江斌^{1, 2},
吴南洋^{1, 2},
陈少莺^{1, 2},
俞伏松^{2, 3, ,}

1.
福建省农业科学院畜牧兽医研究所, 福建福州 350013
2.
福建省畜禽疫病防治工程技术研究中心, 福建福州 350013
3.
福建省农业科学院生物技术研究所, 福建福州 350003

基金项目:

福建省现代农业产业技术体系建设项目 2013-2018

国家现代农业产业技术体系项目 CARS-43

福建省农业科学院院科技创新团队建设项目 2016PI-6

详细信息

作者简介:
程晓霞(1972-), 女, 副研究员, 主要从事动物传染病免疫学研究

通讯作者:
俞伏松(1962-), 男, 研究员, 主要从事动物传染病病原与防治研究(E-mail:chengsy58@163.com)

中图分类号: S852
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- 被引次数: 0
出版历程
- 收稿日期: 2016-12-14
- 修回日期: 2017-07-26
- 刊出日期: 2017-08-28

Isolation and Identification of Duck Plague Virus

CHENG Xiao-xia^{1, 2},
LIN Feng-qiang^{1, 2},
HUANG Mei-qing^{1, 2},
XIAO Shi-feng^{1, 2},
JIANG Bin^{1, 2},
WU Nanyang^{1, 2},
CHEN Shao-ying^{1, 2},
YU Fu-song^{2, 3
, ,}

1.
Institute of Animal Husbandry and Veterinary Medicine, FuJian Academy of Agriculture Sciences, Fuzhou, Fujian 350013, China
2.
Fujian Animal Diseases Control Technology Develppment Center, Fuzhou, Fujian 350013, China
3.
Institute of Biotechnology, Fujian Academy of Agricultural Sciences/Fujian Aquaculture Disease Control and Prevention Center, Fuzhou, Fujian 350003, China

摘要

摘要: 采集疑似鸭瘟病毒自然感染的病死番鸭的肝脾等组织，应用番鸭胚成纤维细胞（MDEF）进行病毒分离，通过对分离毒的血凝特性（HA）测定、间接免疫荧光试验（IFA）荧光定量PCR、PCR产物测序和动物回归试验等初步鉴定。结果显示：通过MDEF从疑似病料中分离到4株病毒（DPVfj1、DPVfj2、DPVfj3、DPVfj4），均不能凝集鸽红细胞；IFA结果排除了分离毒为鹅细小病毒、番鸭细小病毒、鸭呼肠孤病毒、鸭副粘病毒和禽坦布苏病毒；鸭瘟病毒荧光PCR试剂盒检测分离毒核酸均为鸭瘟阳性；鸭瘟病毒（JQ673560）gJ蛋白基因序列特异引物进行PCR扩增均为阳性，且PCR产物序列与鸭瘟病毒参考株gJ蛋白基因序列相似度均大于99%；动物回归试验显示，分离毒人工感染30日龄番鸭和同居感染5日龄雏番鸭均可复制出与自然感染一致的临床表现及病理变化，并能回收到病毒。上述结果表明4株分离毒均为鸭瘟病毒强毒株。
- 鸭瘟病毒 /
- 分离 /
- 鉴定
Abstract: Tissue samples of liver and spleen from the Muscovy ducks that were suspected to have died from the duck plague were collected for this study.Viruses were isolated from the Muscovy duck embryo fibroblasts (MDEF) for a preliminary identification using hemagglutination assay(HA), immunofluorescence analysis(IFA), qPCR, PCR product sequencing, and animal infection test. Four virus strains, DPVfj1, DPVfj2, DPVfj3 and DPVfj4, were thus identified for further investigation. Subsequently, it was found that these strains (a) would not cause red blood cell agglutination on pigeon erythrocytes; (b) were tested negative on IFA with goose parvovirus, Muscovy duck parvovirus, duck reovirus, duck paramyxovirus, and Tembusu virus; (c) showed positive on test with fluorescence RT-PCR kit; (d) had a positive result on their PCR-amplified pair of primers from the specific fragment of gJ protein gene, JQ673560, and a homologygreater than 99% on the sequence of the fragment with that of the duck plague virus(DPV) gJ protein gene; (e)infected 30-day-old ducks by injection and 5-day-old ducklings by co-habitation showing exactly the same clinical symptoms and postmortem signsas in the natural cases; and, (f)were recovered from the diseased birds. The results seemed to verify the fact that DPV caused the duck plaque in natural environment, and that the isolated strains possessed the virulent nature in question.
- duck plague virus /
- isolation /
- identification

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图 1 分离毒致MDEF单层细胞的CPE

注：A为MDEF对照；B为接毒后72 h CPE。

Figure 1. CPE of MDEF monolayer on cells infected by isolated viruses

下载: 全尺寸图片幻灯片

图 2 鸭瘟病毒荧光PCR检测

Figure 2. Result of fluorescence RT PCR detection on DPV

下载: 全尺寸图片幻灯片

图 3 分离毒遗传进化分析

Figure 3. Phylogeny analysis on isolated viruses

下载: 全尺寸图片幻灯片

图 4 人工感染病死番鸭病变

注：1为肝；2为脾；3为肠；4为泄殖腔。

Figure 4. Pathologic changes on Muscovy ducks died from induced infection by isolated viruses

下载: 全尺寸图片幻灯片

参考文献(10)

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