Poliovirus mutant that does not selectively inhibit host cell protein synthesis.

Bernstein, Harris; Sonenberg, Nahum; Baltimore, David

doi:10.1128/mcb.5.11.2913

Cited by 169 publications

(147 citation statements)

References 40 publications

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“…This observation suggests that, far from being a component of the antiviral response in mammalian cells, the dsRNA modifier has a normal cellular function that is inhibited during the antiviral response. Consistent with this idea, the dsRNA modifier was also found to be inhibited during infection with poliovirus, a single-stranded RNA virus whose infection can lead to the accumulation of intracellular dsRNA (6,7,29). The dsRNA modifier was significantly less inhibited during infection with adenovirus, a virus whose virus-associated (VA) RNA products are known to subvert the cellular antiviral response (36).…”

supporting

confidence: 57%

“…Others have shown that some posttranslational components of the cellular response to poly(I -C) are stimulated during poliovirus infection, suggesting that sufficient dsRNA to activate these responses must be present. For 4 example, in HeLa cells infected with a poliovirus mutant defective in the inhibition of cellular translation, viral translation was found to be inhibited eventually by the cell (6). Furthermore, the activation and destabilization of the DAI has been observed during poliovirus infection (7,29).…”

Section: Methodsmentioning

confidence: 99%

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Regulation of a double-stranded RNA modification activity in human cells.

Morrissey¹,

Kirkegaard²

1991

Mol. Cell. Biol.

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A double-stranded RNA (dsRNA)-specffic modification activity from Xenopus oocytes and human cells (dsRNA modifier) converts adenosine residues present in dsRNA to inosines. The function of the dsRNA modifier is unknown, although it has been suggested that it may be part of the cellular antiviral response. We investigated the relationship between the activity of the dsRNA modifier, viral infection, and the antiviral response in human cells induced by poly(rI)-poly(rC) [poly(I C)] treatment. We found, unexpectedly, that treatment of HeLa cells with poly(I. C) or other dsRNA molecules resulted in the dramatic inhibition of the dsRNA modifier. Mixing experiments, reconstruction experiments, and pretreatment of extracts with RNases indicated that inhibition of the dsRNA modifier did not result from the continued presence of a soluble inhibitor (such as dsRNA) in the in vitro modification reactions. Treatment of cells with cyclohexamide or dactinomycin simultaneously with the poly(I C) demonstrated that in vivo inhibition of the dsRNA modifier did not require new transcription or translation. The dsRNA mojification activity was also substantially inhibited in cells infected with poliovirus and was slightly inhibited in cells infected with adenovirus. The inhibition of the dsRNA modifier during the antiviral state is thus not consistent with an antiviral function, and instead suggests another cellular function for dsRNA modification.

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supporting

confidence: 57%

Section: Methodsmentioning

confidence: 99%

Regulation of a double-stranded RNA modification activity in human cells.

Morrissey¹,

Kirkegaard²

1991

Mol. Cell. Biol.

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“…The mutant virus, 3A-2, contains a single amino acid insertion in the 3A coding region (Bernstein et al, 1985). Mutant 3A-2 protein, when expressed in isolation, causes a reduced inhibition of ERto-Golgi traffic compared with wild-type 3A protein (Doedens et al, 1997) and cells infected with 3A-2 mutant virus secrete much higher levels of several cytokines than wild-type-infected cells (Dodd et al, 2001).…”

Section: Fig 6 Characteristics Of Golgi Dispersion During Poliovirumentioning

confidence: 99%

Poliovirus infection blocks ERGIC-to-Golgi trafficking and induces microtubule-dependent disruption of the Golgi complex

Beske

Reichelt

Taylor

et al. 2007

Journal of Cell Science

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Cells infected with poliovirus exhibit a rapid inhibition of protein secretion and disruption of the Golgi complex. Neither the precise step at which the virus inhibits protein secretion nor the fate of the Golgi complex during infection has been determined. We find that transport-vesicle exit from the endoplasmic reticulum (ER) and trafficking to the ER-Golgi intermediate compartment (ERGIC) are unaffected in the poliovirus-infected cell. By contrast, poliovirus infection blocks transport from the ERGIC to the Golgi complex. Poliovirus infection also induces fragmentation of the Golgi complex resulting in diffuse distribution of both large and small vesicles throughout the cell. Pre-treatment with nocodazole prevents complete fragmentation, indicating that microtubules are required for poliovirus-induced Golgi dispersion. However, virally induced inhibition of the secretory pathway is not affected by nocodazole, and Golgi dispersion was found to occur during infection with mutant viruses with reduce ability to inhibit protein secretion. We conclude that the dispersion of the Golgi complex is not in itself the cause of inhibition of traffic between the ERGIC and the Golgi. Instead, these phenomena are independent effects of poliovirus infection on the host secretory complex.

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“…In addition, 17 point mutations in 2A pro were obtained, some of them by site-directed mutagenesis (Y88S, Y88P, and Y88L) and the rest using a recently described genetic system to select cytotoxic-deficient 2A pro mutants in yeast cells (40). Mutant 2A-1 contains a leucine insertion at position 103 as described (44 (Fig. 2).…”

Section: Construction and Expression Of Poliovirus 2amentioning

confidence: 99%