Rapid reconstruction of SARS-CoV-2 using a synthetic genomics platform

被引:0
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作者
Tran Thi Nhu Thao
Fabien Labroussaa
Nadine Ebert
Philip V’kovski
Hanspeter Stalder
Jasmine Portmann
Jenna Kelly
Silvio Steiner
Melle Holwerda
Annika Kratzel
Mitra Gultom
Kimberly Schmied
Laura Laloli
Linda Hüsser
Manon Wider
Stephanie Pfaender
Dagny Hirt
Valentina Cippà
Silvia Crespo-Pomar
Simon Schröder
Doreen Muth
Daniela Niemeyer
Victor M. Corman
Marcel A. Müller
Christian Drosten
Ronald Dijkman
Joerg Jores
Volker Thiel
机构
[1] Institute of Virology and Immunology (IVI),Department of Infectious Diseases and Pathobiology, Vetsuisse Faculty
[2] University of Bern,Graduate School for Biomedical Science
[3] University of Bern,Institute of Veterinary Bacteriology, Vetsuisse Faculty
[4] University of Bern,Insitute for Infectious Diseases
[5] University of Bern,Department for Molecular and Medical Virology
[6] Ruhr-Universität Bochum,Institute of Virology, Charité
[7] corporate member of Freie Universität Berlin,Universitätsmedizin Berlin
[8] Humboldt-Universität zu Berlin,German Centre for Infection Research
[9] and Berlin Institute of Health,Martsinovsky Institute of Medical Parasitology, Tropical and Vector Borne Diseases
[10] associated partner Charité,undefined
[11] Sechenov University,undefined
来源
Nature | 2020年 / 582卷
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摘要
Reverse genetics has been an indispensable tool to gain insights into viral pathogenesis and vaccine development. The genomes of large RNA viruses, such as those from coronaviruses, are cumbersome to clone and manipulate in Escherichia coli owing to the size and occasional instability of the genome1–3. Therefore, an alternative rapid and robust reverse-genetics platform for RNA viruses would benefit the research community. Here we show the full functionality of a yeast-based synthetic genomics platform to genetically reconstruct diverse RNA viruses, including members of the Coronaviridae, Flaviviridae and Pneumoviridae families. Viral subgenomic fragments were generated using viral isolates, cloned viral DNA, clinical samples or synthetic DNA, and these fragments were then reassembled in one step in Saccharomyces cerevisiae using transformation-associated recombination cloning to maintain the genome as a yeast artificial chromosome. T7 RNA polymerase was then used to generate infectious RNA to rescue viable virus. Using this platform, we were able to engineer and generate chemically synthesized clones of the virus, severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2)4, which has caused the recent pandemic of coronavirus disease (COVID-19), in only a week after receipt of the synthetic DNA fragments. The technical advance that we describe here facilitates rapid responses to emerging viruses as it enables the real-time generation and functional characterization of evolving RNA virus variants during an outbreak.
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页码:561 / 565
页数:4
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