A Chikungunya Virus
            <i>trans</i>
            -Replicase System Reveals the Importance of Delayed Nonstructural Polyprotein Processing for Efficient Replication Complex Formation in Mosquito Cells

Bartholomeeusen, Koen; Utt, Age; Coppens, Sandra; Rausalu, Kai; Vereecken, Katleen; Ariën, Kevin K.; Merits, Andres

doi:10.1128/jvi.00152-18

Cited by 38 publications

(60 citation statements)

References 67 publications

(86 reference statements)

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“…Incorporation of one or more reporter-coding sequences into template RNA constructs allows the use of the much more convenient measurement of reporter activities as a proxy for the synthesis of corresponding positive-strand RNAs and is also applicable in a high-throughput format. Therefore, in the current study, as previously (8,36,39), firefly luciferase (Fluc) was used as a substitute for most of the ns ORF and Gaussia luciferase (Gluc) was used as a substitute for the structural ORF in template constructs ( Fig. 1B and 2B).…”

Section: Resultsmentioning

confidence: 99%

“…The effect is due to the high background activity of the reporter resulting from its efficient translation using RNA polymerase II-generated capped transcripts. This activity is often comparable to or even higher than the reporter activity produced from much more abundant viral replicase-generated full-length positive-strand RNAs (36,39).…”

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confidence: 95%

“…In the case of alphaviruses, decoupled replication systems are generally designed to amplify truncated RNA templates where the ns and structural ORFs of alphavirus genome are replaced by sequences encoding different reporter proteins; such systems are often referred to as trans-replication systems. trans-Replication systems have been developed for SINV, SFV, and CHIKV and used to study alphavirus replication complex biogenesis (31)(32)(33) and RNA template sequence requirements (34), for analysis of the impact of template length on the size of replication complexes (35), for tagging of different replicase proteins (36), and for analysis of the impact of different mutations introduced into replicase proteins on viral RNA replication in mammalian (8,37,38) and mosquito (39) cells. While these studies have universally found the alphavirus transreplication systems to be efficient and robust tools, they have also revealed certain technical limitations.…”

mentioning

confidence: 99%

“…While these studies have universally found the alphavirus transreplication systems to be efficient and robust tools, they have also revealed certain technical limitations. Namely, to produce replication-competent template RNA and mRNA for expression of replicase polyproteins, alphavirus trans-replication systems have traditionally used either bacteriophage T7 RNA polymerase and the corresponding promoters (33) or cellular RNA polymerase II promoters, such as the immediate early promoter of human cytomegalovirus (CMV) or the Aedes aegypti polyubiquitin promoter (Ubi) (36,39). The major drawback of the use of bacteriophage T7 RNA polymerase promoters is that the use of such trans-replication systems is restricted to cell lines expressing T7 RNA polymerase, which are generally not available for cell types relevant for in vivo alphavirus infections.…”

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confidence: 99%

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Design and Use of Chikungunya Virus Replication Templates Utilizing Mammalian and Mosquito RNA Polymerase I-Mediated Transcription

Utt

Rausalu

Jakobson

et al. 2019

J Virol

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Chikungunya virus (CHIKV) is a mosquito-borne alphavirus. It has a positive-sense RNA genome that also serves as the mRNA for four nonstructural proteins (nsPs) representing subunits of the viral replicase. Coupling of nsP and RNA synthesis complicates analysis of viral RNA replication. We developed trans-replication systems, where production of replication-competent RNA and expression of viral replicase are uncoupled. Mammalian and mosquito RNA polymerase I promoters were used to produce noncapped RNA templates, which are poorly translated relative to CHIKV replicase-generated capped RNAs. It was found that, in human cells, constructs driven by RNA polymerase I promoters of human and Chinese hamster origin performed equally well. In contrast, RNA polymerase I promoters from Aedes mosquitoes exhibited strong species specificity. In both mammalian and mosquito cells, novel trans-replicase assays had exceptional sensitivity, with up to 105-fold higher reporter expression in the presence of replicase relative to background. Using this highly sensitive assay to analyze CHIKV nsP1 functionality, several mutations that severely reduced, but did not completely block, CHIKV replicase activity were identified: (i) nsP1 tagged at its N terminus with enhanced green fluorescent protein; (ii) mutations D63A and Y248A, blocking the RNA capping; and (iii) mutation R252E, affecting nsP1 membrane anchoring. In contrast, a mutation in the nsP1 palmitoylation site completely inactivated CHIKV replicase in both human and mosquito cells and was lethal for the virus. Our data confirm that this novel system provides a valuable tool to study CHIKV replicase, RNA replication, and virus-host interactions. IMPORTANCE Chikungunya virus (CHIKV) is a medically important pathogen responsible for recent large-scale epidemics. The development of efficient therapies against CHIKV has been hampered by gaps in our understanding of how nonstructural proteins (nsPs) function to form the viral replicase and replicate virus RNA. Here we describe an extremely sensitive assay to analyze the effects of mutations on the virus RNA synthesis machinery in cells of both mammalian (host) and mosquito (vector) origin. Using this system, several lethal mutations in CHIKV nsP1 were shown to reduce but not completely block the ability of its replicase to synthesize viral RNAs. However, in contrast to related alphaviruses, CHIKV replicase was completely inactivated by mutations preventing palmitoylation of nsP1. These data can be used to develop novel, virus-specific antiviral treatments.

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Section: Resultsmentioning

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confidence: 95%

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Design and Use of Chikungunya Virus Replication Templates Utilizing Mammalian and Mosquito RNA Polymerase I-Mediated Transcription

Utt

Rausalu

Jakobson

et al. 2019

J Virol

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“…For this system, one plasmid encodes the CHIKV P1234 polyprotein behind a human cytomegalovirus (hCMV)-driven polymerase II (pol II) promoter, and a second plasmid encodes a pol I promoter-driven viral template RNA for synthesis of luciferase reporters from both the genomic 5′ UTR (firefly luciferase, Fluc) and subgenomic 5′ UTR (Gaussia luciferase, Gluc) by the viral proteins encoded by the P1234 plasmid. The pol II promoter/terminator was substituted for the previously described hCMV-Fluc-Gluc reporter to reduce the background reporter expression (69,71) and improve assay sensitivity. All previously analyzed nsP3 mutations (27) were introduced into viral polymerasecompetent hCMV-P1234 and polymerase-mutated control CMV-P1234 GAA plasmids by site-directed mutagenesis and were transfected into NSC34 cells along with the pol I-Fluc-Gluc template plasmid (Fig.…”

Section: Analysis Of Nsp Function In the Absence Of Virus Infection Umentioning

confidence: 99%

ADP-ribosyl–binding and hydrolase activities of the alphavirus nsP3 macrodomain are critical for initiation of virus replication

Abraham

Hauer

McPherson

et al. 2018

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

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139

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Alphaviruses are plus-strand RNA viruses that cause encephalitis, rash, and arthritis. The nonstructural protein (nsP) precursor polyprotein is translated from genomic RNA and processed into four nsPs. nsP3 has a highly conserved macrodomain (MD) that binds ADP-ribose (ADPr), which can be conjugated to protein as a posttranslational modification involving transfer of ADPr from NAD + by poly ADPr polymerases (PARPs). The nsP3 MD also removes ADPr from mono ADP-ribosylated (MARylated) substrates. To determine which aspects of alphavirus replication require nsP3 MD ADPr-binding and/or hydrolysis function, we studied NSC34 neuronal cells infected with chikungunya virus (CHIKV). Infection induced ADP-ribosylation of cellular proteins without increasing PARP expression, and inhibition of MARylation decreased virus replication. CHIKV with a G32S mutation that reduced ADPr-binding and hydrolase activities was less efficient than WT CHIKV in establishing infection and in producing nsPs, dsRNA, viral RNA, and infectious virus. CHIKV with a Y114A mutation that increased ADPr binding but reduced hydrolase activity, established infection like WT CHIKV, rapidly induced nsP translation, and shut off host protein synthesis with reduced amplification of dsRNA. To assess replicase function independent of virus infection, a transreplicase system was used. Mutant nsP3 MD s D10A, G32E, and G112E with no binding or hydrolase activity had no replicase activity, G32S had little, and Y114A was intermediate to WT. Therefore, ADP ribosylation of proteins and nsP3 MD ADPr binding are necessary for initiation of alphavirus replication, while hydrolase activity facilitates amplification of replication complexes. These observations are consistent with observed nsP3 MD conservation and limited tolerance for mutation. alphavirus | macrodomain | ADP ribosylation | replication complexes | PARP

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Self-amplifying mRNA-Based Vaccine Technology and Its Mode of Action

Maruggi

Ulmer

Rappuoli³

et al. 2021

Current Topics in Microbiology and Immunology

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Self-amplifying mRNAs derived from the genomes of positive-strand RNA viruses have recently come into focus as a promising technology platform for vaccine development. Non-virally delivered self-amplifying mRNA vaccines have the potential to be highly versatile, potent, streamlined, scalable, and inexpensive. By amplifying their genome and the antigen encoding mRNA in the host cell, the self-amplifying mRNA mimics a viral infection, resulting in sustained levels of the target protein combined with self-adjuvanting innate immune responses, ultimately leading to potent and long-lasting antigen-specific humoral and cellular immune responses. Moreover, in principle, any eukaryotic sequence could be encoded by self-amplifying mRNA without the need to change the manufacturing process, thereby enabling a much faster and flexible research and development timeline than the current vaccines and hence a quicker response to emerging infectious diseases. This chapter highlights the rapid progress made in using non-virally delivered self-amplifying mRNA-based vaccines against infectious diseases in animal models. We provide an overview of the unique attributes of this vaccine approach, summarize the growing body of work defining its mechanism of action, discuss the current challenges and latest advances, and highlight perspectives about the future of this promising technology.

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A Chikungunya Virus trans -Replicase System Reveals the Importance of Delayed Nonstructural Polyprotein Processing for Efficient Replication Complex Formation in Mosquito Cells

Cited by 38 publications

References 67 publications

Design and Use of Chikungunya Virus Replication Templates Utilizing Mammalian and Mosquito RNA Polymerase I-Mediated Transcription

Design and Use of Chikungunya Virus Replication Templates Utilizing Mammalian and Mosquito RNA Polymerase I-Mediated Transcription

ADP-ribosyl–binding and hydrolase activities of the alphavirus nsP3 macrodomain are critical for initiation of virus replication

Self-amplifying mRNA-Based Vaccine Technology and Its Mode of Action

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