Rapid Construction of a Replication-Competent Infectious Clone of Human Adenovirus Type 14 by Gibson Assembly

被引:16
作者
Pan, Haibin [1 ]
Yan, Yuqian [1 ]
Zhang, Jing [1 ]
Zhao, Shan [1 ]
Feng, Liqiang [2 ]
Ou, Junxian [1 ]
Cao, Na [1 ]
Li, Min [1 ]
Zhao, Wei [1 ]
Wan, Chengsong [1 ]
Ismail, Ashrafali M. [3 ]
Rajaiya, Jaya [3 ]
Chodosh, James [3 ]
Zhang, Qiwei [1 ]
机构
[1] Southern Med Univ, Sch Publ Hlth, Guangdong Prov Key Lab Trop Dis Res, Guangzhou 510515, Guangdong, Peoples R China
[2] Chinese Acad Sci, Guangzhou Inst Biomed & Hlth, Guangzhou 510530, Guangdong, Peoples R China
[3] Harvard Med Sch, Massachusetts Eye & Ear, Howe Lab, Dept Ophthalmol, Boston, MA 02114 USA
来源
VIRUSES-BASEL | 2018年 / 10卷 / 10期
基金
中国国家自然科学基金;
关键词
Human adenovirus type 14; infectious clone; Gibson Assembly; ACUTE RESPIRATORY-DISEASE; GENOME SEQUENCE; NEUTRALIZING ANTIBODIES; MILITARY RECRUITS; VIRUS; DNA; OUTBREAK; VECTOR; RECOMBINANT; GENERATION;
D O I
10.3390/v10100568
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
In 1955, Human adenovirus type 14 (HAdV-B14p) was firstly identified in a military trainee diagnosed as acute respiratory disease (ARD) in the Netherlands. Fifty years later, a genomic variant, HAdV-B14p1, re-emerged in the U.S. and caused large and fatal ARD outbreaks. Subsequently, more and more ARD outbreaks occurred in Canada, the UK, Ireland, and China, in both military and civil settings. To generate a tool for the efficient characterization of this new genomic variant, a full-length infectious genomic clone of HAdV-B14 was successfully constructed using one-step Gibson Assembly method in this study. Firstly, the full genome of HAdV-B14p1 strain GZ01, the first HAdV-B14 isolate in China, was assembled into pBR322 plasmid by Gibson Assembly. The pBRAdV14 plasmid, generated by Gibson Assembly, was analyzed and verified by PCR, restriction enzymes digestion and the sequencing. Secondly, viruses were rescued from pBRAdV14-transfected A549 cells. The integrity of the rescued viruses was identified by restriction enzyme analysis. The complete sequence of the infectious clone was further sequenced. No mutation was found in the infectious clone during the construction when compared with the parental virus and pBR322 sequences. The direct immunofluorescence assay indicated the expression of the hexon protein. Finally, typical virions were observed; the one-step growth curves further showed that the DNA replication and viral reproduction efficiency of pBRAd14 derived viruses was similar with that of wild-type HAdV-B14 strain. The successful construction of the replication-competent infectious clone of pBRAdV14 facilitates the development of vaccine and antiviral drugs against HAdV-B14, as well as provides a novel strategy for rapid construction of infectious viral clones for other large-genome DNA viruses.
引用
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页数:16
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