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| 减蛋综合征病毒末端片段的克隆及细胞内DNA重组 | |
| 引用本文: | 向华,章金刚,宣华,李茂祥,王国庆,刘振润,万遂如.减蛋综合征病毒末端片段的克隆及细胞内DNA重组[J].中国兽医学报,1999,19(3):226-229. |
| 作者姓名: | 向华 章金刚 宣华 李茂祥 王国庆 刘振润 万遂如 |
| 作者单位: | 1. 解放军农牧大学兽医学院,长春,130062 2. Jinlin International Enconomical and Technological Corporation 3. 吉林省国际经济技术合作公司 |
| 基金项目: | 国家自然科学基金,农业部重点资助 |
| 摘 要: | 采用9~10日龄非免疫鸭胚增殖的减蛋综合征病毒(EDSV)AA-2毒株,经差速离心法浓缩纯化后,提取病毒基因组DNA。采用碱变性法除去病毒基因组共价结合的末端蛋白(TP)。用限制性内切酶HindⅢ水解纯化的EDSV基因组DNA。经低熔点琼脂糖凝胶电泳后,回收C、D、E片段。克隆到pUC19载体的HindⅢ和SmaⅠ双酶切位点及HindⅢ位点上,经蓝白斑筛选和单、双酶切鉴定,获得了pUHC、pUHD、pUHE重组质粒,其中pUHC含有末端片段。将EDSVSalⅠ水解产生并回收的大片段与pUHC在95℃水浴中变性,65℃复性后,用钙离子介导法,共转染50%~70%的单层鸭胚成纤维细胞,转染后36h开始产生细胞病变(CPE)。48h后将病变细胞反复冻融,经尿囊腔接种9~10日龄鸭胚,回收的尿囊液能凝集鸡红细胞,这种血凝性能被EDSV高免血清抑制,电镜下观察到腺病毒样颗粒。 |
| 关 键 词: | 减蛋综合征病毒 末端蛋白 末端片段 重组DNA |
Cloning of the Terminal Fragment of EDSV and the DNA Recombination in vivo |
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| Xiang Hua,Zhang Jingang,Xuan Hua,Li Maoxiang,Wang Guoqing,Liu Zhenrun,Wan Shuiru.Cloning of the Terminal Fragment of EDSV and the DNA Recombination in vivo[J].Chinese Journal of Veterinary Science,1999,19(3):226-229. | |
| Authors: | Xiang Hua Zhang Jingang Xuan Hua Li Maoxiang Wang Guoqing Liu Zhenrun Wan Shuiru |
| Abstract: | Egg drop syndrome virus (EDSV)AA2 strain was purified from the duck embryo allantonic fluids using differential centrifugation. The typical adenovirus virons were observed under electron microscope.The viral DNA that was prepared and purified showed a clear band about 33 kb in agarose gel electrophoresis. The terminal peptides(TP) were removed with alkaline treatment.Then the EDSV DNA was digested by Hind .The C,D,E fragments were retook,and cloned into pUC19 between Hind and Sma sites.The mixture of recombinant plasmid and the leftend fragment of viral DNA digested by Sal ,were denatured at 95 for 10 min and annealed at 65 for 30 min, then cotransfected into duck embryo fibroblast of 50p% confluent cells in 35 mm well by Ca2 reagent .The typical cytopathic effects(CPE) were observed at 36 h later,in contrast, Cla fragment or recombinant plasmid did not make the DEF pathic .The medium was passaged in 9or 10dayold embryonated eggs by allantonic cavity inoculation and the allantonic fluid havested was tested by HA with HI and adenoviruslike virons were also found using electron microscope.This research established a method for the aviadenovirus vector constructing at the right region of EDSV genomic DNA. |
| Keywords: | egg drop syndrome virus terminal protein terminal fragment recombinant DNA |
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