COVID-19 Collection

Journal article

Rapid cloning-free mutagenesis of new SARS-CoV-2 variants using a novel reverse genetics platform

Abstract:: Reverse genetic systems enable the engineering of RNA virus genomes and are instrumental in studying RNA virus biology. With the recent outbreak of the coronavirus disease 2019 pandemic, already established methods were challenged by the large genome of severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2). Herein we present an elaborated strategy for the rapid and straightforward rescue of recombinant plus-stranded RNA viruses with high sequence fidelity using the example of SARS-CoV-2. The strategy called CLEVER (CLoning-free and Exchangeable system for Virus Engineering and Rescue) is based on the intracellular recombination of transfected overlapping DNA fragments allowing the direct mutagenesis within the initial PCR-amplification step. Furthermore, by introducing a linker fragment - harboring all heterologous sequences - viral RNA can directly serve as a template for manipulating and rescuing recombinant mutant virus, without any cloning step. Overall, this strategy will facilitate recombinant SARS-CoV-2 rescue and accelerate its manipulation. Using our protocol, newly emerging variants can quickly be engineered to further elucidate their biology. To demonstrate its potential as a reverse genetics platform for plus-stranded RNA viruses, the protocol has been successfully applied for the cloning-free rescue of recombinant Chikungunya and Dengue virus.

Publication status:: Published

Peer review status:: Peer reviewed

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APA Style

Kipfer, E. T., Hauser, D., Lett, M. J., Otte, F., Urda, L., Zhang, Y., Lang, C. M. R., Chami, M., Mittelholzer, C., & Klimkait, T. (2023). Rapid cloning-free mutagenesis of new SARS-CoV-2 variants using a novel reverse genetics platform. ELife, 12, RP89035.

MLA Style

Kipfer, ET, et al. “Rapid Cloning-Free Mutagenesis of New SARS-CoV-2 Variants Using a Novel Reverse Genetics Platform.” ELife, vol. 12, 2023, p. RP89035.

Chicago Style

Kipfer, ET, D Hauser, MJ Lett, et al. 2023. “Rapid Cloning-Free Mutagenesis of New SARS-CoV-2 Variants Using a Novel Reverse Genetics Platform.” ELife 12: RP89035.
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Files:: Kipfer_et_al_2023_Rapid_cloning-free_mutagenesis.pdf

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Publisher copy:: 10.7554/elife.89035

Authors

+ Kipfer, ET More by this author

Role:: Author
ORCID:: 0000-0001-5870-6784

+ Hauser, D More by this author

Role:: Author
ORCID:: 0000-0001-9950-365X

+ Lett, MJ More by this author

Institution:: University of Oxford
Role:: Author
ORCID:: 0000-0002-7230-9264

+ Otte, F More by this author

Role:: Author
ORCID:: 0000-0003-0572-617X

+ Urda, L More by this author

Role:: Author
ORCID:: 0009-0007-4122-515X

More authors...

Publisher:: eLife Sciences Publications
Journal:: eLife More from this journal
Volume:: 12
Pages:: RP89035
Publication date:: 2023-08-11
DOI:: 10.7554/elife.89035
EISSN:: 2050-084X
ISSN:: 2050-084X

Language:: English
Keywords:: Genome

Gene

Virology

Infectious disease (medical specialty)

Computational biology

Coronavirus disease 2019 (COVID-19)

Cloning (programming)

Synthetic biology

Coronavirus

Genetics

Reverse genetics

RNA

Virus

Biology
Pubs id:: 2358566
Local pid:: pubs:2358566
Source identifiers:: W4385759524
Deposit date:: 2026-04-23
ARK identifier:: ark:/29072/ora_414481938711493e8fd8dd598c4c3311

Terms of use

Copyright date:: 2023

Licence:: CC Attribution (CC BY)

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