| Literature DB >> 26831931 |
Changping Xu1, Hualei Wang2,3, Hongli Jin2,4, Na Feng2,3, Xuexing Zheng2,3, Zengguo Cao2, Ling Li2, Jianzhong Wang2,5, Feihu Yan2, Lina Wang2, Hang Chi2, Weiwei Gai2, Chong Wang2, Yongkun Zhao2, Yan Feng1, Tiecheng Wang2, Yuwei Gao2,3, Yiyu Lu6, Songtao Yang7,8, Xianzhu Xia9,10.
Abstract
Ebola virus (species Zaire ebolavirus) (EBOV) is highly virulent in humans. The largest recorded outbreak of Ebola hemorrhagic fever in West Africa to date was caused by EBOV. Therefore, it is necessary to develop a detection method for this virus that can be easily distributed and implemented. In the current study, we developed a visual assay that can detect EBOV-associated nucleic acids. This assay combines reverse transcription loop-mediated isothermal amplification and nucleic acid strip detection (RT-LAMP-NAD). Nucleic acid amplification can be achieved in a one-step process at a constant temperature (58 °C, 35 min), and the amplified products can be visualized within 2-5 min using a nucleic acid strip detection device. The assay is capable of detecting 30 copies of artificial EBOV glycoprotein (GP) RNA and RNA encoding EBOV GP from 10(2) TCID50 recombinant viral particles per ml with high specificity. Overall, the RT-LAMP-NAD method is simple and has high sensitivity and specificity; therefore, it is especially suitable for the rapid detection of EBOV in African regions.Entities:
Mesh:
Substances:
Year: 2016 PMID: 26831931 DOI: 10.1007/s00705-016-2763-5
Source DB: PubMed Journal: Arch Virol ISSN: 0304-8608 Impact factor: 2.574