Activation of RNase L is dependent on OAS3 expression during infection with diverse human viruses

Li, Yize; Banerjee, Shuvomoy; Wang, Yuyan; Goldstein, Stephen A.; Dong, Bin; Gaughan, Christina; Silverman, Robert H.; Weiss, Susan R.

doi:10.1073/pnas.1519657113

Cited by 215 publications

(287 citation statements)

References 48 publications

Supporting

Mentioning

267

Contrasting

Order By: Relevance

“…First, we examined RV-1B replication in human bronchial epithelial cells during a single replication cycle by infecting all cells in the monolayer, using a high multiplicity of infection (MOI,20). After inoculation, medium was added and plates containing multiple replicate wells of infected cells were incubated at 33°C or 37°C.…”

Section: Resultsmentioning

confidence: 99%

“…These include protein kinase R (PKR), a dsRNA-dependent enzyme that halts protein synthesis upon dsRNA detection, and 2′5′ oligoadenylate synthetases (OAS). Upon binding of dsRNA, OAS enzymes OAS1-OAS3 generate oligomers of adenosine from ATP that then activate the RNAdegrading enzyme RNAseL, leading to degradation of viral RNA (19)(20)(21). Even though PKR, RNAseL, and OAS genes are ISGs (expression is enhanced by IFN signaling), they can also be constitutively expressed.…”

Section: Rnasel Replication and Cell Death Kinetics Restrict Rv At Comentioning

confidence: 99%

See 1 more Smart Citation

Two interferon-independent double-stranded RNA-induced host defense strategies suppress the common cold virus at warm temperature

Foxman

Storer

Vanaja

et al. 2016

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

View full text Add to dashboard Cite

Most strains of rhinovirus (RV), the common cold virus, replicate better at cool temperatures found in the nasal cavity (33-35°C) than at lung temperature (37°C). Recent studies found that although 37°C temperature suppressed RV growth largely by engaging the type 1 IFN response in infected epithelial cells, a significant temperature dependence to viral replication remained in cells devoid of IFN induction or signaling. To gain insight into IFN-independent mechanisms limiting RV replication at 37°C, we studied RV infection in human bronchial epithelial cells and H1-HeLa cells. During the single replication cycle, RV exhibited temperature-dependent replication in both cell types in the absence of IFN induction. At 37°C, earlier signs of apoptosis in RV-infected cells were accompanied by reduced virus production. Furthermore, apoptosis of epithelial cells was enhanced at 37°C in response to diverse stimuli. Dynamic mathematical modeling and B cell lymphoma 2 (BCL2) overexpression revealed that temperature-dependent host cell death could partially account for the temperature-dependent growth observed during RV amplification, but also suggested additional mechanisms of virus control. In search of a redundant antiviral pathway, we identified a role for the RNA-degrading enzyme RNAseL. Simultaneous antagonism of apoptosis and RNAseL increased viral replication and dramatically reduced temperature dependence. These findings reveal two IFN-independent mechanisms active in innate defense against RV, and demonstrate that even in the absence of IFNs, temperature-dependent RV amplification is largely a result of host cell antiviral restriction mechanisms operating more effectively at 37°C than at 33°C. apoptosis | RNaseL | innate immunity | rhinovirus | respiratory immunity I n the 1960s, rhinoviruses (RVs) were first cultured from patient samples and shown to cause acute upper respiratory infections (a.k.a. common colds). Early work showed that RV isolates replicated best in culture when incubated at temperatures slightly cooler than core body temperature (33-35°C) (1, 2). This observation fit with the role of RV as a cause of disease in the nasal cavity, but not the lungs, as the nasal cavity is cooled by inhalation of environmental air, but the lungs are generally considered to be at core body temperature (37°C). The primary target cells of RV infection are the airway epithelial cells that line the respiratory tract. Similar to all cells of the body, airway epithelial cells are equipped with a cell-intrinsic innate immune system that can sense the presence of a viral infection, using pattern recognition receptors such as toll-like receptors (TLRs) and RIG-I like receptors (RLRs), and can respond to the infection by inducing antiviral effector mechanisms (3). Recently, we used mouse primary airway cells and a mouse-adapted RV to show that replicating RV is recognized by the RLRs within airway epithelial cells, leading to two innate immune signaling events that occur more robustly at warm temperature than at cool temperatu...

show abstract

Section: Resultsmentioning

confidence: 99%

Section: Rnasel Replication and Cell Death Kinetics Restrict Rv At Comentioning

confidence: 99%

Two interferon-independent double-stranded RNA-induced host defense strategies suppress the common cold virus at warm temperature

Foxman

Storer

Vanaja

et al. 2016

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

View full text Add to dashboard Cite

show abstract

“…Pathogenic viruses may also share receptors or intracellular proteins/pathways also required by other viruses, thereby reducing their availability for viral replication. Innate antiviral responses may also be induced by potentially "protective" viruses that increase resistance to high-level replication by pathogenic viruses in the same (sapelovirus versus enterovirus) or different (parvovirus versus enterovirus) viral families (73)(74)(75)(76)(77)(78).…”

Section: Discussionmentioning

confidence: 99%

Case-Control Comparison of Enteric Viromes in Captive Rhesus Macaques with Acute or Idiopathic Chronic Diarrhea

Kapusinszky

Ardeshir

Mulvaney

et al. 2017

J Virol

View full text Add to dashboard Cite

Diarrhea is the major cause of non-research-associated morbidity and mortality affecting the supply of rhesus macaques and, potentially, their responses to experimental treatments. Idiopathic chronic diarrhea (ICD) in rhesus macaques also resembles ulcerative colitis, one form of human inflammatory bowel disease. To test for viral etiologies, we characterized and compared the fecal viromes from 32 healthy animals, 31 animals with acute diarrhea, and 29 animals with ICD. The overall fractions of eukaryotic viral reads were 0.063% for the healthy group, 0.131% for the acute-diarrhea group, and 0.297% for the chronic-diarrhea group. Eukaryotic viruses belonging to 6 viral families, as well as numerous circular Rep-encoding singlestranded DNA (CRESS DNA) viral genomes, were identified. The most commonly detected sequences were from picornaviruses, making up 59 to 88% of all viral reads, followed by 9 to 17% for CRESS DNA virus sequences. The remaining 5 virus families, Adenoviridae, Astroviridae, Anelloviridae, Picobirnaviridae, and Parvoviridae, collectively made up 1 to 3% of the viral reads, except for parvoviruses, which made up 23% of the viral reads in the healthy group. Detected members of the families Picornaviridae and Parvoviridae were highly diverse, consisting of multiple genera, species, and genotypes. Coinfections with members of up to six viral families were detected. Complete and partial viral genomes were assembled and used to measure the number of matching short sequence reads in feces from the 92 animals in the two clinical and the healthy control groups. Several enterovirus genotypes and CRESS DNA genomes were associated with ICD relative to healthy animals. Conversely, higher read numbers from different parvoviruses were associated with healthy animals. Our study reveals a high level of enteric coinfections with diverse viruses in a captive rhesus macaque colony and identifies several viruses positively or negatively associated with ICD.KEYWORDS enterovirus, sapelovirus, parvovirus, CRESS-DNA, idiopathic diarrhea, rhesus macaques, enteric disease etiology W e compared the enteric viromes of captive rhesus macaques (Macaca mulatta) with acute and idiopathic chronic diarrhea (ICD) to those of healthy animals using a case-control study. The genomes of several known and new viruses were characterized using metagenomics. We showed that some specific enterovirus genotypes and some small circular DNA genomes are associated with chronic idiopathic diarrhea, providing candidates for further testing of their pathogenicity. Other viruses, including some parvoviruses, were found at significantly higher levels in healthy animals.

show abstract

“…It is interesting that cytosolic viral RNA can also serve as cGAS activating ligand by forming DNA: RNA hybrid . In general, it should be noted that some viral RNA intermediately transcribed from the cytoplasmic genome of a DNA virus can be also be recognized by cytosolic RNA sensors . Moreover, DNA reverse transcribed from genomic RNA of retroviruses can be recognized by cytosolic DNA sensors …”

Section: Pattern Recognition Receptors For Viral Nucleic Acidsmentioning

confidence: 99%

“…All members of the family are cytosolic viral RNA sensors that are functionally activated by viral dsRNAs and transcriptionally activated by type 1 IFNs . During viral infection, OAS3 activates latent RNase L (Figure ), whereas OAS 1 and OAS2 have other antiviral functions . Without OAS3 activation, RNase L does not sense viral RNAs .…”

Section: Pattern Recognition Receptors For Viral Nucleic Acidsmentioning

confidence: 99%

Defects in interferon pathways as potential biomarkers of sensitivity to oncolytic viruses

Matveeva

Chumakov

2018

Reviews in Medical Virology

View full text Add to dashboard Cite

Increased sensitivity of cancer cells to viruses is a prerequisite for the success of oncolytic virotherapy. One of the major causes of such a phenotype is the disruption of innate antiviral defenses associated with dysfunction of type 1 interferons (IFNs) that permits unlimited replication of viruses in cancer cells. Defects in IFN pathways help cancer progression by providing additional advantages to tumor cells. However, while these defects promote the survival and accelerated proliferation of malignant cells, they facilitate viral replication and thus enhance the efficiency of viral oncolysis. This review describes a broad spectrum of defects in genes that participate in IFN induction and IFN response pathways. Expression levels and/or functional activities of these genes are frequently low or absent in cancer cells, making them sensitive to virus infection. Therefore, certain specific defects in IFN signaling cascades might serve as potential biomarkers to help in identifying individual cancer patients who are likely to benefit from oncolytic virotherapy.

show abstract

Activation of RNase L is dependent on OAS3 expression during infection with diverse human viruses

Cited by 215 publications

References 48 publications

Two interferon-independent double-stranded RNA-induced host defense strategies suppress the common cold virus at warm temperature

Two interferon-independent double-stranded RNA-induced host defense strategies suppress the common cold virus at warm temperature

Case-Control Comparison of Enteric Viromes in Captive Rhesus Macaques with Acute or Idiopathic Chronic Diarrhea

Defects in interferon pathways as potential biomarkers of sensitivity to oncolytic viruses

Contact Info

Product

Resources

About