| 鸭胚成纤维细胞中鸭瘟强毒的增殖特性研究 |
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| 引用本文: | 郭宇飞,程安春,汪铭书,贾仁勇,文明,周伟光,周毅,陈孝跃.鸭胚成纤维细胞中鸭瘟强毒的增殖特性研究[J].病毒学报,2008,24(5):352-357. |
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| 作者姓名: | 郭宇飞 程安春 汪铭书 贾仁勇 文明 周伟光 周毅 陈孝跃 |
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| 作者单位: | 四川农业大学,动物医学院,禽病防治研究中心,四川,雅安,625014;动物疫病与人类健康四川省重点实验室,四川,雅安,625014;动物疫病与人类健康四川省重点实验室,四川,雅安,625014;动物疫病与人类健康四川省重点实验室,四川,雅安,625014;贵州大学,动物科学学院,贵州,贵阳,550025;动物疫病与人类健康四川省重点实验室,四川,雅安,625014;内蒙古农业大学,动物科学与医学学院,内蒙古,呼和浩特,010018;四川农业大学,动物医学院,禽病防治研究中心,四川,雅安,625014 |
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| 基金项目: | 国家自然科学基金,国家科技支撑计划,科技部农业科技成果转化基金,高校科技创新工程项目,教育部跨世纪优秀人才培养计划,四川省应用基础研究计划,中国博士后科学基金 |
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| 摘 要: | 通过细胞培养物光学显微观察、细胞超薄切片研究、定量PCR检测技术对鸭胚成纤维细胞中鸭瘟强毒的增殖特性进行了研究.结果表明:鸭瘟强毒接种鸭胚成纤维细胞后42 h,可使细胞培养物出现大量明显的蚀斑病变.细胞培养物的超薄切片电镜观察研究表明,病毒核酸在胞核内常集中分布,呈直径35~45 nm的圆形颗粒状;核衣壳在胞核和胞浆内都有分布,呈直径90~100 nm的网形颗粒状;成熟病毒位于胞浆空泡内,呈直径150~300 nm的圆形,有囊膜和皮层结构;病毒通过囊膜与胞膜融合入侵细胞,在核内生成核酸、装配核衣壳,在胞浆中得到皮层,出芽到胞浆空泡内获得囊膜,通过胞吐作用释放到胞外.定量PCR研究表明:鸭瘟强毒接种细胞后10 h开始明显复制,接毒后30 h时含量趋于稳定,接毒后22 h时开始向胞外释放,50 h时达最大值,细胞和上清中病毒含量的增幅均为103左右,病毒主要存在于细胞中,其含量为上清的102~103倍.
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| 关 键 词: | 鸭瘟强毒 鸭胚成纤维细胞 蚀斑 电镜 定量PCR |
Studies on the Proparagation Characteristics of Duck Plague Virulent Virus in Duck Embryo Fibroblasts |
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| GUO Yu-fei,CHENG An-chun,WANG Ming-shu,JIA Ren-yong,WEN Ming,ZHOU Wei-guang,ZHOU Yi,CHEN Xiao-yue.Studies on the Proparagation Characteristics of Duck Plague Virulent Virus in Duck Embryo Fibroblasts[J].Chinese Journal of Virology,2008,24(5):352-357. |
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| Authors: | GUO Yu-fei CHENG An-chun WANG Ming-shu JIA Ren-yong WEN Ming ZHOU Wei-guang ZHOU Yi CHEN Xiao-yue |
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| Abstract: | The propagation characteristics of virulent duck plague virus(DPV)in duck embryo fibroblast(DEF)were studied by the method of light microscopy observation of DEF cell culture monolayer,electron microscopy observation of infected DEF cell culture,real-time PCR detecting virus propagation.The results demonstrated that on duck embryo fibroblast a number of plaques were formed by DPV 42 h postinfection.Electron microscopy of the ultrathin section of infected duck embryo fibroblasts demonstrated that the nucleic acid of DPV was round in shape with diameter of 35~45 nm and was often in a cluster in the nucleus of DEF.The nucleocapsid of DPV was round in shape with diameter of 90~100 nm and could be observed both in nucleus and cytoplasm of DEF.The mature DPV which had the structures of envelop and tegument was spherical in shape with diameter of 150~300 nm and was located in cytoplasmic vacuoles.DPV penetrated the DEF cell membrane by direct fusion between the viral envelop and the plasma membrane.Progeny viral nucleic acid was produced in the nucleus and the assembled nucleocapsids obtained the structure of tegument in the cytoplasm and obtained the structure of envelop by budding into the cytoplasmic vesicles.The mature DPV particles were released out of the cell through exocytosis of the cytoplasmic vesicles.Detection of DPV by real-time PCR demonstrated that virus in DEF began its obvious propagation 10 h postinfection and virus amount tended to increase until 30 h postinfection.DPV began to be released into the supernatant 22 h postinfection and the DPV amount peaked 50 h postinfection,when the virus content in DEF and supernatant both underwent approximately 103 fold increase.DPV mainly existed in the DEF and the virus content in DEF was 102~103 fold than the supernatant. |
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| Keywords: | virulent duck plague virus duck embryo fibroblasts plaque electron microscopy real-time PCR |
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