| 稳定表达呼吸道合胞病毒非结构蛋白NS1细胞的构建及其生物特性研究 |
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| 引用本文: | 秦笙,王玉涛,杨子峰,陈俏连,关文达,伍时冠,刘文宽,郑兆广,李海涛,周荣.稳定表达呼吸道合胞病毒非结构蛋白NS1细胞的构建及其生物特性研究[J].病毒学报,2011,27(6):587-593. |
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| 作者姓名: | 秦笙 王玉涛 杨子峰 陈俏连 关文达 伍时冠 刘文宽 郑兆广 李海涛 周荣 |
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| 作者单位: | 广州呼吸疾病研究所 呼吸疾病国家重点实验室(广州医学院),广东省 广州市,510230;广州呼吸疾病研究所 呼吸疾病国家重点实验室(广州医学院),广东省 广州市 510230;广州呼研所医药科技有限公司,广东省 广州市 510663;澳门科技大学中医药学院,中国澳门特别行政区;广州呼研所医药科技有限公司,广东省 广州市,510663;澳门科技大学中医药学院,中国澳门特别行政区;广州呼吸疾病研究所 呼吸疾病国家重点实验室(广州医学院),广东省 广州市 510230;广州呼研所医药科技有限公司,广东省 广州市 510663 |
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| 基金项目: | 澳门科学技术发展基金会,039/2009/A;广州市科技支撑计划项目,2010J-E401;广州市医药卫生科技项目,2008-YB-146 |
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| 摘 要: | 获得稳定表达RSV病毒NS1基因的HEp-2-NS1细胞株并对其生物学特性进行初步研究。采用RT-PCR方法从RSV病毒中获得NS1全长基因,克隆到逆转录病毒载体pBABE-puro中,重组载体与包装质粒PIK通过磷酸钙共沉淀法转染包装细胞293FT细胞,产生的逆转录病毒颗粒感染HEp-2细胞,经嘌呤霉素筛选后得到稳定表达细胞株,用QPCR、细胞病变染色法、RT-PCR和间接免疫荧光法检测细胞中NS1 mRNA和蛋白表达情况。结果表明重组逆转录病毒载体pBABE-NS1经双酶切及测序鉴定正确;筛选获得5株阳性单克隆细胞株,QPCR结果显示HEp-2-NS1细胞有NS1基因扩增,其中d株的相对表达量是正常细胞对照组的8 483倍;在外源干扰素作用下,HEp-2-NS1细胞仍对VSV病毒保持敏感,细胞感染病毒48h后染色结果显示全部死亡;对第3代及第30代细胞的RT-PCR和间接免疫荧光法检测结果显示,导入的NS1基因在HEp-2细胞中不仅能转录成相应的mRNA而且能成功稳定地表达。成功构建了稳定表达RSV病毒非结构蛋白NS1的HEp-2-NS1改造细胞株,为建立适用于临床分离的转基因细胞提供良好的基础。
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| 关 键 词: | 呼吸道合胞病毒 非结构蛋白 细胞 |
Development and characterization of a stable cell line expressing respiratory syncytial virus non-structural protein NS1 |
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| Qin Sheng,Wang Yu-Tao,Yang Zi-Feng,Chen Qiao-Lian,Guan Wen-Da,Wu Shi-Guan,Liu Wen-Kuan,Zhen Zhao-Guang,Li Hai-Tao,Zhou Rong.Development and characterization of a stable cell line expressing respiratory syncytial virus non-structural protein NS1[J].Chinese Journal of Virology,2011,27(6):587-593. |
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| Authors: | Qin Sheng Wang Yu-Tao Yang Zi-Feng Chen Qiao-Lian Guan Wen-Da Wu Shi-Guan Liu Wen-Kuan Zhen Zhao-Guang Li Hai-Tao Zhou Rong |
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| Institution: | Guangzhou Institute of Respiratory Disease, State Key Laboratory of Respiratory Diseases, Guangzhou Medical University, Guangzhou 510230, China. b96106@163.com |
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| Abstract: | To develop a stable cell line that could express the RSV NS1, the full-length RSV NS1 gene was generated by RT-PCR amplification from respiratory syncytial virus. NS1 gene was ligated with pBABE-puro to construct the recombinant retroviral expression plasmid pBABE-NS1, which was cotransfected into 293FT packaging cells with PIK packaging plasmid by calcium phosphate co-precipitation. The supernatant of 293FT was collected to infect HEp-2 cells, the resulting cell clones stably expressing NS1 were screened by puromycin. Using QPCR, CPE staining method and indirect immunofluorescence assay, the expression of NS1 at both gene and protein levels was identified. The recombinant plasmid pBABE-NS1 was identified by EcoRI and BamHI endonuclease digestion and the sequence analysis. QPCR results showed that the NS1 gene amplification in HEp-2-NS1 cells was 8483 fold higher than that in HEp-2 cells. Although the exogenous interferon was added, all cells were destroyed after 48 hours post infection using CPE staining method, showing that HEp-2-NS1 cells remained sensitive to the VSV virus. The results of RT-PCR and indirect immunofluorescence assay showed that the NS1 gene in HEp-2 cells could not only transcribe mRNA, but also express NS1 protein steadily. We had successfully established HEp-2-NS1 cell lines with stable expression of respiratory syncytial virus non-structural protein NS1. |
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