Reverse genetics with a full-length infectious cDNA of severe acute respiratory syndrome coronavirus

Yount, Boyd; Curtis, Kristopher M.; Fritz, Elizabeth A.; Hensley, Lisa E.; Jahrling, Peter B.; Prentice, Erik; Denison, Mark R.; Geisbert, Thomas W.; Baric, Ralph S.

doi:10.1073/pnas.1735582100

Cited by 350 publications

(413 citation statements)

References 46 publications

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“…DNA fragments were isolated from 1.0% agarose gels with the Qiaquick gel extraction kit (Qiagen) and visualized by using Dark Reader technology (Clare Chemical Research, Denver, CO). The six subgenomic cDNA clones (A-F) span the SARS-CoV genome (9). ORF 7a͞b, located within SARS F (nt 27273-27772), was replaced with the Renilla luciferase gene as described with GFP in ref.…”

Section: Construction Of Renilla Luciferase Encoding Sars-cov Recombimentioning

confidence: 99%

“…The SARS full-length cDNA was assembled, and full-length transcripts were synthesized and mixed with polyadenylated N gene transcripts and then electroporated into cells (9,40). Viruses were plaque-purified in Vero E6 cells, and stock was grown in 75-cm 2 flasks.…”

Section: Construction Of Sars Plasmids Containing Redesigned Trs Circmentioning

confidence: 99%

“…ORFs 2-8 are encoded in subgenomic mRNAs (mRNAs 2-9) synthesized as a nested set of 3Ј coterminal molecules. Leader RNA sequences, encoded at the 5Ј end of the genome, are joined to body sequences at distinct transcription regulatory sequences (TRSs) that contain the core sequence ACGAAC (7,9). SARS-CoV likely uses transcription attenuation to synthesize both full-and subgenomic-length negative strand RNAs containing antileader sequences, which then function as the templates for the synthesis of like-sized mRNAs (10,11).…”

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Rewiring the severe acute respiratory syndrome coronavirus (SARS-CoV) transcription circuit: Engineering a recombination-resistant genome

Yount

Roberts

Lindesmith

et al. 2006

Proc. Natl. Acad. Sci. U.S.A.

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Live virus vaccines provide significant protection against many detrimental human and animal diseases, but reversion to virulence by mutation and recombination has reduced appeal. Using severe acute respiratory syndrome coronavirus as a model, we engineered a different transcription regulatory circuit and isolated recombinant viruses. The transcription network allowed for efficient expression of the viral transcripts and proteins, and the recombinant viruses replicated to WT levels. Recombinant genomes were then constructed that contained mixtures of the WT and mutant regulatory circuits, reflecting recombinant viruses that might occur in nature. Although viable viruses could readily be isolated from WT and recombinant genomes containing homogeneous transcription circuits, chimeras that contained mixed regulatory networks were invariantly lethal, because viable chimeric viruses were not isolated. Mechanistically, mixed regulatory circuits promoted inefficient subgenomic transcription from inappropriate start sites, resulting in truncated ORFs and effectively minimize viral structural protein expression. Engineering regulatory transcription circuits of intercommunicating alleles successfully introduces genetic traps into a viral genome that are lethal in RNA recombinant progeny viruses.regulation ͉ systems biology ͉ vaccine design L ive virus vaccines represent a crucial intervention strategy that has been documented to improve the overall health of populations. Concerns regarding reversion to virulence by mutation and recombination, coupled with the associated challenges in developing these vaccines commercially, have diminished the appeal of live virus vaccines (1, 2). The dichotomy between the well known protective efficacy and the costs and risks of developing live virus vaccines has been recognized as a Grand Challenge in Global Health by the National Foundation for Infectious Diseases, which has called for new methods to prevent reversion or recombination repair.Severe acute respiratory syndrome coronavirus (SARS-CoV) emerged suddenly and spread worldwide in 2003, causing Ϸ800 deaths (3). Zoonotic SARS-CoV strains, common in farm animals and bats, dictate a need for continued surveillance and the development of efficacious vaccines (4, 5). SARS-CoV is a tractable system for innovative live virus vaccine design because the pathogen is highly virulent and replicates efficiently in animal models, and a robust reverse genetic system is available. Importantly, CoVs undergo RNA recombination events at high frequency, and recombination-mediated vaccine failures in animals are a problem (6).SARS-CoV contains a positive, single-stranded, Ϸ29,700-nt RNA genome bound by the nucleocapsid protein (N) and an envelope containing the S, ORF3a, E, and M structural proteins. The SARS-CoV genome contains nine ORFs, and ORF1 encodes the viral replicase proteins that are required for subgenomic and genome-length RNA synthesis (7). Downstream of ORF1 and interspaced among the structural genes are the unique SARS-CoV group-specif...

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Section: Construction Of Renilla Luciferase Encoding Sars-cov Recombimentioning

confidence: 99%

Section: Construction Of Sars Plasmids Containing Redesigned Trs Circmentioning

confidence: 99%

mentioning

confidence: 99%

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Rewiring the severe acute respiratory syndrome coronavirus (SARS-CoV) transcription circuit: Engineering a recombination-resistant genome

Yount

Roberts

Lindesmith

et al. 2006

Proc. Natl. Acad. Sci. U.S.A.

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“…Besides containing RNA-dependent RNA polymerase, RNA helicase, and proteases (4,12,15,23,37), which are all common to positive-strand RNA viruses, the CoV replicase was recently predicted to contain a variety of RNA-processing enzymes that are extremely rare or absent in other RNA viruses, including endoribonuclease (NendoU), 3Ј-to-5Ј exoribonuclease (ExoN), 2Ј-O-ribose methyltransferase (2Ј-O-MT), ADP ribose 1ЈЈ-phosphatase, and, in a subset of group 2 coronaviruses, cyclic phosphodiesterase (25, 36). These enzymatic activities might be involved in the replication of the largest known RNA virus genome and in the production of an extensive set of 5Ј-and 3Ј-coterminal subgenomic RNAs (11,14,25,36).The study of CoV molecular biology has been profoundly advanced by the recent construction of full-length cDNA clones (3,6,26,27,(32)(33)(34) and self-replicating RNAs, or replicons (2,28,30). Due to the large size of the CoV RNA genome and the instability of some CoV replicase gene sequences in bacteria, cDNA clones and replicons have been engineered using bacterial artificial chromosomes (BACs) (3), in vitro ligation of CoV cDNA fragments (32), and vaccinia virus as a vector for the propagation of CoV full-length cDNAs (27).…”

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confidence: 99%

Construction of a Severe Acute Respiratory Syndrome Coronavirus Infectious cDNA Clone and a Replicon To Study Coronavirus RNA Synthesis

Almazán

DeDiego

Galán

et al. 2006

J Virol

208

284

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The engineering of a full-length infectious cDNA clone and a functional replicon of the severe acute respiratory syndrome coronavirus (SARS-CoV) Urbani strain as bacterial artificial chromosomes (BACs) is described in this study. In this system, the viral RNA was expressed in the cell nucleus under the control of the cytomegalovirus promoter and further amplified in the cytoplasm by the viral replicase. Both the infectious clone and the replicon were fully stable in Escherichia coli. Using the SARS-CoV replicon, we have shown that the recently described RNA-processing enzymes exoribonuclease, endoribonuclease, and 2-O-ribose methyltransferase were essential for efficient coronavirus RNA synthesis. The SARS reverse genetic system developed as a BAC constitutes a useful tool for the study of fundamental viral processes and also for developing genetically defined vaccines.The etiologic agent causing severe acute respiratory syndrome (SARS) is a novel coronavirus (CoV) (8,10,(16)(17)(18)21). This virus causes a life-threatening respiratory disease for which no fully efficacious therapy is available. SARS-CoV is a member of group 2 of the Coronaviridae family within the order Nidovirales (13), which is composed of enveloped, singlestranded, positive-sense RNA viruses relevant in animal and human health (5, 9). Two-thirds of the 29.7-kb SARS-CoV genome carries the replicase gene, which comprises two overlapping open reading frames, ORF 1a and ORF 1b, the latter being translated by a ribosomal frameshift mechanism (29). Translation of both ORFs results in the synthesis of two polyproteins that are processed by viral proteinases to release the components of the replication-transcription complex (36,37). Besides containing RNA-dependent RNA polymerase, RNA helicase, and proteases (4,12,15,23,37), which are all common to positive-strand RNA viruses, the CoV replicase was recently predicted to contain a variety of RNA-processing enzymes that are extremely rare or absent in other RNA viruses, including endoribonuclease (NendoU), 3Ј-to-5Ј exoribonuclease (ExoN), 2Ј-O-ribose methyltransferase (2Ј-O-MT), ADP ribose 1ЈЈ-phosphatase, and, in a subset of group 2 coronaviruses, cyclic phosphodiesterase (25, 36). These enzymatic activities might be involved in the replication of the largest known RNA virus genome and in the production of an extensive set of 5Ј-and 3Ј-coterminal subgenomic RNAs (11,14,25,36).The study of CoV molecular biology has been profoundly advanced by the recent construction of full-length cDNA clones (3,6,26,27,(32)(33)(34) and self-replicating RNAs, or replicons (2,28,30). Due to the large size of the CoV RNA genome and the instability of some CoV replicase gene sequences in bacteria, cDNA clones and replicons have been engineered using bacterial artificial chromosomes (BACs) (3), in vitro ligation of CoV cDNA fragments (32), and vaccinia virus as a vector for the propagation of CoV full-length cDNAs (27). Recently, a SARS-CoV full-length cDNA clone has been generated by the approach of using the in vitro li...

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“…Genetic obstacles were obliterated by Thiel et al (11), who developed the first molecular clone for a HCoV, HCoV-229E, after inserting a full-length genome copy into a poxvirus vector to drive full-length infectious transcripts. Shortly thereafter, Yount et al (12) isolated a molecular clone of the SARSCoV by cloning the genome as six fragments that could be systematically assembled into a full-length cDNA in vitro and serve as the genomic template for the recovery of infectious transcripts (12). Using genetic approaches, the role of the accessory genes in coronavirus pathogenesis has been studied, foreign genes have been expressed, and coronavirus replicon particles have been developed as delivery vehicles for heterologous vaccines and therapeutics (13).…”

Section: Hcovsmentioning

confidence: 99%

Humanized mice develop coronavirus respiratory disease

Baric

Sims

2005

Proc. Natl. Acad. Sci. U.S.A.

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Reverse genetics with a full-length infectious cDNA of severe acute respiratory syndrome coronavirus

Cited by 350 publications

References 46 publications

Rewiring the severe acute respiratory syndrome coronavirus (SARS-CoV) transcription circuit: Engineering a recombination-resistant genome

Rewiring the severe acute respiratory syndrome coronavirus (SARS-CoV) transcription circuit: Engineering a recombination-resistant genome

Construction of a Severe Acute Respiratory Syndrome Coronavirus Infectious cDNA Clone and a Replicon To Study Coronavirus RNA Synthesis

Humanized mice develop coronavirus respiratory disease

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