scholarly journals Rolling Circle Amplification is a high fidelity and efficient alternative to plasmid preparation for the rescue of infectious clones

2020 ◽  
Author(s):  
Jeffrey M. Marano ◽  
Christina Chuong ◽  
James Weger-Lucarelli
Keyword(s):  
Cdna Clone ◽  
Plasmid Dna ◽  
Viral Genome ◽  
Traditional Approach ◽  
Rolling Circle Amplification ◽  
Infectious Cdna Clone ◽  
Cdna Clones ◽  
High Fidelity ◽  
Rolling Circle ◽  
Viral Yield

AbstractAlphaviruses (genus Alphavirus; family Togaviridae) are a medically relevant family of viruses that include chikungunya virus, Eastern equine encephalitis virus, and the emerging Mayaro virus. Infectious cDNA clones of these viruses are necessary molecular tools to understand viral biology and to create effective vaccines. The traditional approach to rescuing virus from an infectious cDNA clone requires propagating large amounts of plasmids in bacteria, which can result in unwanted mutations in the viral genome due to bacterial toxicity or recombination and requires specialized equipment and knowledge to propagate the bacteria. Here, we present an alternative to the bacterial-based plasmid platform that uses rolling circle amplification (RCA), an in vitro technology that amplifies plasmid DNA using only basic equipment. We demonstrate that the use of RCA to amplify plasmid DNA is comparable to the use of a midiprepped plasmid in terms of viral yield, albeit with a slight delay in virus recovery kinetics. RCA, however, has lower cost and time requirements and amplifies DNA with high fidelity and with no chance of unwanted mutations due to toxicity. We show that sequential RCA reactions do not introduce mutations into the viral genome and, thus, can replace the need for glycerol stocks or bacteria entirely. These results indicate that RCA is a viable alternative to traditional plasmid-based approaches to viral rescue.ImportanceThe development of infectious cDNA clones is critical to studying viral pathogenesis and for developing vaccines. The current method for propagating clones in bacteria is limited by the toxicity of the viral genome within the bacterial host, resulting in deleterious mutations in the viral genome, which can only be detected through whole-genome sequencing. These mutations can attenuate the virus, leading to lost time and resources and potentially confounding results. We have developed an alternative method of preparing large quantities of DNA that can be directly transfected to recover infectious virus without the need for bacteria by amplifying the infectious cDNA clone plasmid using rolling circle amplification (RCA). Our results indicate that viral rescue from an RCA product produces a viral yield equal to bacterial-derived plasmid DNA, albeit with a slight delay in replication kinetics. The RCA platform, however, is significantly more cost and time-efficient compared to traditional approaches. When the simplicity and costs of RCA are combined, we propose that a shift to an RCA platform will benefit the field of molecular virology and could have significant advantages for recombinant vaccine production.

scholarly journals Recovery of Virulent and RNase-Negative Attenuated Type 2 Bovine Viral Diarrhea Viruses from Infectious cDNA Clones

2002 ◽  
Vol 76 (16) ◽  
pp. 8494-8503 ◽  
Author(s):  
Christiane Meyer ◽  
Martina von Freyburg ◽  
Knut Elbers ◽  
Gregor Meyers
Keyword(s):  
Cdna Clone ◽  
Infectious Cdna Clone ◽  
Wild Type Virus ◽  
Bovine Viral Diarrhea ◽  
Cdna Clones ◽  
Wild Type ◽  
Viral Glycoprotein ◽  
Diarrhea Virus ◽  
Viral Diarrhea

ABSTRACT Cloned cDNA derived from the genome of the virulent type 2 bovine viral diarrhea virus (BVDV) strain NY'93/C was sequenced and served for establishment of the infectious cDNA clone pKANE40A. Virus recovered from pKANE40A exhibited growth characteristics similar to those of wild-type BVDV NY'93/C and proved to be clinically indistinguishable from the wild-type virus in animal experiments. A virus mutant in which the RNase residing in the viral glycoprotein Erns was inactivated, revealed an attenuated phenotype. The plasmid pKANE40A represents the first infectious cDNA clone established for a type 2 BVDV and offers a variety of new approaches to analyze the mechanisms of BVDV-induced disease in cattle.

scholarly journals Direct retransformation of yeast with plasmid DNA isolated from single yeast colonies using rolling circle amplification

BioTechniques ◽  
2003 ◽  
Vol 35 (4) ◽  
pp. 774-779 ◽  
Author(s):  
Xiaodong Ding ◽  
Anita K. Snyder ◽  
Regina Shaw ◽  
William G. Farmerie ◽  
Wen-Yuan Song
Keyword(s):  
Plasmid Dna ◽  
Rolling Circle Amplification ◽  
Rolling Circle

scholarly journals Genome Sequence, Full-Length Infectious cDNA Clone, and Mapping of Viral Double-Stranded RNA Accumulation Determinant of Hypovirus CHV1-EP721

2006 ◽  
Vol 81 (4) ◽  
pp. 1813-1820 ◽  
Author(s):  
Haiyan Lin ◽  
Xiuwan Lan ◽  
Hong Liao ◽  
Todd B. Parsley ◽  
Donald L. Nuss ◽  
...  
Keyword(s):  
Genome Sequence ◽  
Cdna Clone ◽  
Amino Acid Level ◽  
Cryphonectria Parasitica ◽  
Infectious Cdna Clone ◽  
Full Length ◽  
Cdna Clones ◽  
Coding Region ◽  
Viral Dsrna ◽  
Double Stranded Rna

ABSTRACT Cryphonectria parasitica strain EP721 is infected with a strain of hypovirus CHV1, CHV1-EP721, and exhibits typical hypovirulence-associated traits such as reduced pigmentation and reduced asexual sporulation. However, the accumulation of the viral double-stranded RNA (dsRNA) in this hypovirus-infected C. parasitica strain is atypically low. We now report the complete nucleotide sequence and construction of a full-length infectious cDNA clone for hypovirus CHV1-EP721. The genome sequence of CHV1-EP721 was determined to be 12,724 bp in length and to share extensive homology with two other hypovirus strains, CHV1-Euro7 and CHV1-EP713, with an average of 99% and 90% identities at the nucleotide level and 99% and 92% identities at the amino acid level, respectively. CHV1-EP721 was successfully introduced into virus-free fungal host strain EP721(-v) by transfection with transcripts derived from a full-length viral cDNA. The transfected strain had a phenotype indistinguishable from that of EP721, and the accumulation of CHV1-EP721 dsRNA in the transfectant was lower than those transfected by CHV1-Euro7 and CHV1-EP713 transcripts. Through the construction of chimeric viruses by domain swapping using infectious cDNA clones of CHV1-EP721, CHV1-EP713, and CHV1-Euro7 hypoviruses, the determinant for the low level of viral dsRNA accumulation in CHV1-EP721 was mapped to the second of two CHV1-EP721 open reading frames (ORFs), ORF B. Further refined swapping of domains within ORF B identified a 2.5-kb coding region between p48 and the polymerase domain of CHV1-EP721 as being responsible for the low viral dsRNA accumulation. Evidence is also provided that low rates of hypovirus transmission through conidial spores correlates with low viral dsRNA accumulation.

scholarly journals Replication, Integration, and Packaging of Plasmid DNA following Cotransfection with Baculovirus Viral DNA

1999 ◽  
Vol 73 (7) ◽  
pp. 5473-5480 ◽  
Author(s):  
Yuntao Wu ◽  
Ge Liu ◽  
Eric B. Carstens
Keyword(s):  
Dna Replication ◽  
Plasmid Dna ◽  
Viral Genome ◽  
Serial Passage ◽  
Viral Dna ◽  
Common Procedure ◽  
Rolling Circle ◽  
Large Deletions ◽  
Putative Origin ◽  
Integration Sites

ABSTRACT Infection-dependent replication assays have been used to identify numerous putative origins of baculovirus replication. However, plasmid DNA, when cotransfected into insect cells with Autographa californica multinucleocapsid nucleopolyhedrovirus (AcMNPV) DNA, replicates independently of any viral sequence in cis (11). Cotransfection of transfer plasmids and baculovirus DNA is a common procedure used in generating recombinant viruses and in measuring the level of gene expression in transient-expression assays. We have examined the fate of a series of vector plasmids in cotransfection experiments. The data reveal that these plasmids replicate following cotransfection and the replication of plasmid DNA is not due to acquisition of viral putative origin sequences. The conformation of plasmid DNA replicating in the cotransfected cells was analyzed and found to exist as high-molecular-weight concatemers. Ten to 25% of the replicated plasmid DNA was integrated into multiple locations on the viral genome and was present in progeny virions following serial passage. Sequence analysis of plasmid-viral DNA junction sites revealed no homologous or conserved sequences in the proximity of the integration sites, suggesting that nonhomologous recombination was involved during the integration process. These data suggest that while a rolling-circle mechanism could be used for baculovirus DNA replication, recombination may also be involved in this process. Plasmid integration may generate large deletions of the viral genome, suggesting that the process of DNA replication in baculovirus may be prone to generation of defective genomes.

scholarly journals Infectious cDNA clone of the hepatitis C virus genotype 1 prototype sequence

2001 ◽  
Vol 82 (6) ◽  
pp. 1291-1297 ◽  
Author(s):  
Robert E. Lanford ◽  
Helen Lee ◽  
Deborah Chavez ◽  
Bernadette Guerra ◽  
Kathleen M. Brasky
Keyword(s):  
Hepatitis C Virus ◽  
Hepatitis C ◽  
Cdna Clone ◽  
Infectious Cdna Clone ◽  
Full Length ◽  
Cdna Clones ◽  
Amino Acid Residues ◽  
Genotype 1 ◽  
Virus Genotype ◽  
Hcv Genotype 1

A full-length cDNA clone of the hepatitis C virus (HCV) genotype 1 prototype (subtype 1a) sequence was constructed. Synthetic RNA produced from the initial cDNA clone was not infectious following intrahepatic inoculation of a chimpanzee. A consensus clone was prepared by comparison with multiple full-length HCV sequences of genotypes 1, 2 and 3. A total of 11 non-consensus amino acid residues were altered by mutagenesis. Synthetic RNA from the repaired clone initiated a typical, acute-resolving HCV infection following intrahepatic inoculation of a chimpanzee. In addition, at least one of three chimeric cDNA clones constructed between the HCV-1 and H77 genotype 1a strains of HCV was infectious in a chimpanzee. This is the first example of an infectious chimeric HCV clone. An infectious cDNA clone of HCV-1 will be of particular value, since it is the prototype HCV sequence and many commonly used reagents are based on this sequence.

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