检索规则说明:AND代表“并且”;OR代表“或者”;NOT代表“不包含”;(注意必须大写,运算符两边需空一格)
检 索 范 例 :范例一: (K=图书馆学 OR K=情报学) AND A=范并思 范例二:J=计算机应用与软件 AND (U=C++ OR U=Basic) NOT M=Visual
名 称:
注 释:
作 者:潘兹书[1] 张楚瑜[1] 陈玉栋[1] 闵平[1]
出 处:《武汉大学学报(理学版)》2002年第4期466-470,共5页Journal of Wuhan University:Natural Science Edition
基 金:湖北省科技攻关重点项目资助
摘 要:将以PRVgG为启动子 ,SV4 0polyA为加尾信号的CSFVE2表达盒克隆于包含伪狂犬病病毒 (PRV)tk基因和gH基因片段的重组质粒pTK2 .5 ,替换掉tk基因的SalⅠ与XhoⅠ酶切位点之间的序列 ,构建了携带CSFVE2基因的转移载体pTKE2 免疫荧光检测证实 ,转染BHK2 1细胞的pTKE2在感染PRV的情况下 ,能表达E2蛋白 采用特异性引物PCR方法扩增gfp表达盒 ,对酶切位点进行改造 ,将其克隆到pTKE2的SalⅠ位点 ,构建了用PRVgG启动子和HCMVIE启动子分别控制E2基因和gfp基因表达、两基因取向相反的双基因转移载体pTKE2 .GFP 将双基因转移载体pTKE2 .GFP转染BHK2 1细胞中 ,12h后在荧光显微镜下观察到呈绿色荧光的GFP表达 。The E2 gene of CSFV was inserted downstream of the promoter of PRV gG gene, and upstream of SV40 polyadenylation signal, and an E2 gene expression cassette was constructed. The tk gene sequence between Sal Ⅰ and Xho Ⅰ sites of the plasmid pTK2.5 containing the complete tk gene and partial gH gene of PRV was replaced by the E2 gene expression cassette, which resulted in a recombinant PRV transfer vector pTKE2. Transient expression of E2 from pTKE2 was identified by immuno\|fluroscence staining. A green flurocence protein gene ( gfp ) expression cassette was amplificated by PCR with the modified flanking sites to insert it in plasmid pTKE2. The gfp expression cassette was cloned into Sal Ⅰ site of pTKE2, and the resulted coexpression vector was named as pTKE2.GFP, and expression of E2 and gfp genes were controlled by the PRV gG and HCMV IE promoters, respectively. These two promoters were oriented in opposite directions to prevent the possibility of polarity effects. pTKE2.GFP was transfected into BHK21 cells, and GFP expression could be detected in the transfected cells as 12 h post\|transfection. These results might be contributive to the development of an genetically engineered PRV bivalent marker vaccine.
分 类 号:S852.65[农业科学—基础兽医学]
正在载入数据...
正在载入数据...
正在载入数据...
正在载入数据...
正在载入数据...
正在载入数据...
正在载入数据...
正在链接到云南高校图书馆文献保障联盟下载...
云南高校图书馆联盟文献共享服务平台 版权所有©
您的IP:216.73.216.117