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构建并表征一种具有复制能力的基于3型人腺病毒的载体,作为一种活疫苗候选物和病毒递送载体。

Construction and characterization of a replication-competent human adenovirus type 3-based vector as a live-vaccine candidate and a viral delivery vector.

作者信息

Zhang Qiwei, Su Xiaobo, Seto Donald, Zheng Bo-Jian, Tian Xingui, Sheng Huiying, Li Haitao, Wang Youshao, Zhou Rong

机构信息

Central Laboratory, Guangzhou Children's Hospital, 318 Renmin Zhong Road, Guangzhou 510120, China.

出版信息

Vaccine. 2009 Feb 18;27(8):1145-53. doi: 10.1016/j.vaccine.2008.12.039. Epub 2009 Jan 13.

Abstract

In southern China, as well as in neighboring Asian regions, human adenovirus type 3 (HAdV-3) outbreaks have become very prevalent in recent years. To address this problem regionally and globally, a recombinant virus has been constructed, containing a full-length infectious genomic clone of HAdV-3, to act as a vaccine. This was constructed by using a bacterial homologous recombination mechanism and was based on the cloning, manipulation and maintenance of the full-length adenovirus genome as a stable plasmid in E. coli. The resultant recombinant viral DNA was screened, identified and characterized by duplex PCR, Western blot, indirect immunofluorescence assay and electron microscopy. This putative vaccine strain was shown to be fully infectious in permissive cells, and no genome mutations were found in the recombinant plasmid. To demonstrate the utility of such a vaccine, a recombinant HAdV-3 plasmid expressing the reporter molecule eGFP was also constructed. This confirmed the recombinant protein expression capability. Mice immunized with this recombinant eGFP adenovirus by either intramuscular injection, intragastric or intranasal inoculation routes raised a significant antibody response to eGFP. Our results have provided a solid foundation for development of a recombinant live vaccine and potential more effective adenovirus vector-based delivery system for immune and gene therapy.

摘要

在中国南方以及亚洲周边地区,近年来人类3型腺病毒(HAdV-3)暴发变得极为普遍。为了在区域和全球范围内解决这一问题,已构建了一种重组病毒,其包含HAdV-3的全长感染性基因组克隆,用作疫苗。这是通过细菌同源重组机制构建的,基于将全长腺病毒基因组作为稳定质粒在大肠杆菌中进行克隆、操作和保存。通过双链PCR、蛋白质印迹法、间接免疫荧光测定和电子显微镜对所得重组病毒DNA进行筛选、鉴定和表征。该推定疫苗株在允许细胞中显示出完全感染性,并且在重组质粒中未发现基因组突变。为了证明这种疫苗的效用,还构建了表达报告分子eGFP的重组HAdV-3质粒。这证实了重组蛋白表达能力。通过肌肉注射、胃内或鼻内接种途径用这种重组eGFP腺病毒免疫的小鼠对eGFP产生了显著的抗体反应。我们的结果为开发重组活疫苗以及潜在的更有效的基于腺病毒载体的免疫和基因治疗递送系统提供了坚实基础。

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