Rapid Recovery of Classical Swine Fever Virus Directly from Cloned cDNA

文献类型: 外文期刊

第一作者: Huang Jun-hua

作者: Huang Jun-hua;Li Yong-feng;He Fan;Li Dan;Sun Yuan;Han Wen;Qiu Hua-ji

作者机构:

关键词: classical swine fever virus;reverse genetics;T7 RNA polymerase;stable cell line

期刊名称:JOURNAL OF INTEGRATIVE AGRICULTURE ( 影响因子:2.848; 五年影响因子:2.979 )

ISSN: 2095-3119

年卷期: 2013 年 12 卷 5 期

页码:

收录情况: SCI

摘要: The reverse genetics for classical swine fever virus (CSFV) is currently based on the transfection of in vitro transcribed RNA from a viral genomic cDNA clone, which is inefficient and time-consuming. This study was aimed to develop an improved method for rapid recovery of CSFV directly from cloned cDNA. Full-length genomic cDNA from the CSFV Shimen strain, which was flanked by a T7 promoter, the hepatitis delta virus ribozyme and T7 terminator sequences, was cloned into the low-copy vector pOK12, producing pOKShimen-RzT Phi. Direct transfection of pOKShimen-RzT Phi into PK/T7 cells, a PK-15-derived cell line stably expressing bacteriophage T7 RNA polymerase, allowed CSFV to be rescued rapidly and efficiently, i.e., at least 12 h faster and 31.6-fold greater viral titer when compared with the in vitro transcription-based rescue system. Furthermore, the progeny virus rescued from PK/T7 cells was indistinguishable, both in vitro and in vivo, from its parent virus and the virus rescued from classical reverse genetics. The reverse genetics based on intracellular transcription is efficient, convenient and cost-effective. The PK/T7 cell line can be used to rescue CSFV directly from cloned cDNA and it can also be used as an intracellular transcription and expression system for studying the structure and function of viral genes.

分类号:

  • 相关文献

[1]Characterization of a pathogenic full-length cDNA clone of a virulent porcine epidemic diarrhea virus strain AH2012/12 in China. Fan, Baochao,Yu, Zhengyu,Pang, Fengjiao,Xu, Xiangwei,Zhang, Baimeng,Guo, Rongli,He, Kongwang,Li, Bin,Fan, Baochao,Yu, Zhengyu,Pang, Fengjiao,Xu, Xiangwei,Zhang, Baimeng,Guo, Rongli,He, Kongwang,Li, Bin.

[2]Generation and evaluation of a genetically attenuated Newcastle disease virus rGM-VIIm as a genotype-matched vaccine. Sun, Minhua,Xiang, Bin,Li, Yaling,Xie, Peng,Gao, Shimin,Kang, Yinfeng,Gao, Pei,Li, Yanling,Wang, Zhaoxiong,Liang, Jianpeng,Yu, Deshui,Ren, Tao,Sun, Minhua,Xiang, Bin,Li, Yaling,Xie, Peng,Gao, Shimin,Kang, Yinfeng,Gao, Pei,Li, Yanling,Wang, Zhaoxiong,Liang, Jianpeng,Yu, Deshui,Ren, Tao,Sun, Minhua,Xiang, Bin,Li, Yaling,Xie, Peng,Gao, Shimin,Kang, Yinfeng,Gao, Pei,Li, Yanling,Wang, Zhaoxiong,Liang, Jianpeng,Yu, Deshui,Ren, Tao,Sun, Minhua,Xiang, Bin,Li, Yaling,Xie, Peng,Gao, Shimin,Kang, Yinfeng,Gao, Pei,Li, Yanling,Wang, Zhaoxiong,Liang, Jianpeng,Yu, Deshui,Ren, Tao,Sun, Minhua,Gao, Shimin,Kang, Yinfeng,Wang, Zhaoxiong.

[3]Efficacy of a high-yield attenuated vaccine strain wholly derived from avian influenza viruses by use of reverse genetics. Liu, Ming,Liu, Ming.

[4]Alternative reverse genetics system for influenza viruses based on a synthesized swine 45S rRNA promoter. Wang, Kai,Huang, Qi,Yang, Zhiwei,Qi, Kezong,Chen, Hongjun,Wang, Kai,Huang, Qi,Yang, Zhiwei,Liu, Hongmei,Chen, Hongjun.

[5]Infective viruses produced from full-length complementary DNA of swine vesicular disease viruses HK/70 strain. Zheng Haixue,Liu Xinagtao,Shang Youjun,Wu Jinyan,Bai Xingwen,Jin Ye,Sun Shiqi,Guo Huichen,Tian Hong,Feng Xia,Yin Shaunghui,Guo Jianhong,Cong Guozheng,Liu Zaixin,Chang Huiyun,Ma Junwu,Xie Qingge.

[6]Functional analysis of GUS expression patterns and T-DNA integration characteristics in rice enhancer trap lines. Peng, H,Huang, HM,Yang, YZ,Zhai, Y,Wu, JX,Huang, DF,Lu, TG.

[7]Generation by reverse genetics of an effective attenuated Newcastle disease virus vaccine based on a prevalent highly virulent Chinese strain. Liu, Meng-Meng,Cheng, Jin-Long,Yu, Xiao-Hui,Zhang, Guo-Zhong,Qin, Zhuo-Ming,Tian, Fu-Lin.

[8]Recovery of infectious type Asia1 foot-and-mouth disease virus from suckling mice directly inoculated with an RNA polymerase I/II-driven unidirectional transcription plasmid. Lian, Kaiqi,Yang, Fan,Zhu, Zixiang,Cao, Weijun,Jin, Ye,Li, Dan,Zhang, Keshan,Guo, Jianhong,Zheng, Haixue,Liu, Xiangtao.

[9]Development of a reverse genetics system based on RNA polymerase II for Newcastle disease virus genotype VII. Wang, Jianzhong,Yin, Renfu,Cong, Yanlong,Ding, Zhuang,Wang, Chunfeng,Feng, Na,Wang, Hualei,Zheng, Xuexing,Yang, Songtao,Gao, Yuwei,Xia, Xianzhu,Liu, Xiufan,Hu, Shunlin,Ding, Chan,Yu, Shengqing.

[10]The deletion of an extra six nucleotides in the 5 '-untranslated region of the nucleoprotein gene of Newcastle disease virus NA-1 decreases virulence. Liu, Jiaxu,Cong, Yanlong,Yin, Renfu,Ding, Zhuang,Wang, Chunfeng,Wang, Chunfeng,Ding, Chan,Yu, Shengqing,Liu, Xiufan. 2014

[11]A reassortment vaccine candidate as the improved formulation to induce protection against very virulent infectious bursal disease virus. Qi, Xiaole,Chen, Yuming,Ren, Xiangang,Zhang, Lizhou,Gao, Li,Wang, Nian,Qin, Liting,Wang, Yongqiang,Gao, Yulong,Wang, Xiaomei. 2014

[12]Rescue of virulent class I Newcastle disease virus variant 9a5b-D5C1. Yu, Yang,Qiu, Xusheng,Xu, Dan,Zhan, Yuan,Meng, Chunchun,Wei, Nana,Chen, Hongjun,Tan, Lei,Yu, Shengqing,Ding, Chan,Ding, Chan,Yu, Yang,Liu, Xiufan,Qin, Aijian. 2012

[13]Porcine reproductive and respiratory syndrome virus as a vector: Immunogenicity of green fluorescent protein and porcine circovirus type 2 capsid expressed from dedicated subgenomic RNAs. Du, Yijun,Song, Cheng,Yoo, Dongwan,Pei, Yanlong,Hodgins, Douglas C.,Wu, Jiaqiang,Song, Cheng,Welch, Siao-Kun W.,Calvert, Jay G.,Li, Gang. 2009

[14]An improved method for infectious bursal disease virus rescue using RNA polymerase II system. Qi, Xiaole,Gao, Wong,Gao, Honglei,Deng, Xiaoyun,Bu, Zhigao,Wang, Xiaoyan,Fu, Chaoyang,Wang, Xiaomei. 2007

[15]Development of a tailored vaccine against challenge with very virulent infectious bursal disease virus of chickens using reverse genetics. Gao, Li,Qi, Xiaole,Li, Kai,Gao, Honglei,Gao, Yulong,Qin, Liting,Wang, Yongqiang,Wang, Xiaomei. 2011

[16]Protective efficacy of a high-growth reassortant swine H3N2 inactivated vaccine constructed by reverse genetic manipulation. Wen, Feng,Ma, Ji-Hong,Yu, Hai,Yang, Fu-Ru,Huang, Meng,Zhou, Yan-Jun,Li, Ze-Jun,Tong, Guang-Zhi.

[17]Progress of reverse genetics technique in influenza virus. Liu Da-Fei,Liu Chun-Guo,Liu Ming,Liu Da-Cheng. 2008

[18]Down-regulation of cellular protein heme oxygenase 1 inhibits proliferation of classical swine fever virus in PK-15 cells. Shi, Zixue,Guo, Huancheng,Yang, Zhi,Tu, Changchun,Shi, Zixue,Ma, Zhiyong,Sun, Jinfu.

[19]Enhanced expression of the E-rns protein of classical swine fever virus in yeast and its application in an indirect enzyme-linked immunosorbent assay for antibody differentiation of infected from vaccinated animals. Luo, Yuzi,Li, Lin,Dong, Mei,Xu, Jingjing,Shao, Lina,Lei, Jianlin,Li, Na,He, Wen-Rui,Zhao, Bibo,Li, Su,Li, Yongfeng,Sun, Yuan,Qiu, Hua-Ji,Austermann-Busch, Sophia,Becher, Paul,Liu, Lihong,Luo, Yuzi,Li, Lin,Xu, Jingjing,Shao, Lina,Lei, Jianlin,He, Wen-Rui,Zhao, Bibo,Li, Su,Li, Yongfeng,Liu, Lihong,Sun, Yuan,Qiu, Hua-Ji.

[20]Development of a triplex TaqMan real-time RT-PCR assay for differential detection of wild-type and HCLV vaccine strains of classical swine fever virus and bovine viral diarrhea virus 1. Zhang, Xing-Juan,Han, Qiu-Ying,Sun, Yuan,Zhang, Xin,Qiu, Hua-Ji.

作者其他论文 更多>>

微信小程序