Interferon inhibits Sendai virus-induced cell fusion: an effect on cell membrane fluidity.

Chatterjee, Sabyasachi; Cheung, Herbert C.; Hunter, Eric

doi:10.1073/pnas.79.3.835

Cited by 43 publications

(24 citation statements)

References 30 publications

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“…Inhibition was maximum at 24 h after treatment with 1,000 U of interferon per ml and was dose dependent and reversible with time. Pinocytosis was inhibited when human and chicken embryo cells were treated with homologous, but not heterologous, interferons.In addition to inhibiting viral replication, interferon treatment of cells produces a variety of effects on the plasma membrane (2,3,7,9,12,15) 91:238a, 1981) reported that interferon treatment of thioglycollate-elicited mouse peritoneal macrophages caused a marked change in the distribution of microtubules and 10-nm filaments in a major fraction of the cells; this alteration was correlated with an inhibition of pinocytosis. The results reported here describe some details of the inhibition of pinocytosis in cells treated with interferon.…”

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confidence: 99%

Interferon treatment inhibits pinocytosis.

Wilcox¹,

Whitaker-Dowling²,

Youngner³

et al. 1983

Mol. Cell. Biol.

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Treating mouse L cells with crude or purified mouse interferon inhibited fluidphase pinocytosis. Inhibition was maximum at 24 h after treatment with 1,000 U of interferon per ml and was dose dependent and reversible with time. Pinocytosis was inhibited when human and chicken embryo cells were treated with homologous, but not heterologous, interferons.In addition to inhibiting viral replication, interferon treatment of cells produces a variety of effects on the plasma membrane (2,3,7,9,12,15) 91:238a, 1981) reported that interferon treatment of thioglycollate-elicited mouse peritoneal macrophages caused a marked change in the distribution of microtubules and 10-nm filaments in a major fraction of the cells; this alteration was correlated with an inhibition of pinocytosis. The results reported here describe some details of the inhibition of pinocytosis in cells treated with interferon.Mouse L cells were pretreated with 1,000 U of crude mouse interferon per ml for 24 h before the uptake of horseradish peroxidase (HRP) was measured. Untreated control cells and interferon-treated cells both internalized HRP at a rate which was linear with respect to time and to the HRP concentration in the medium (Fig. 1A and B). However, the rate of HRP uptake in the interferon-treated cells was only about 20% of the control rate (Fig. 1A). The uptake of fluorescein-dextran was also inhibited, and examination by fluorescence microscopy (8) suggested that all the cells in the population were inhibited to a similar extent (data not shown).To determine whether interferon treatment inhibits pinocytosis by altering the interaction between pinocytic vesicles and lysosomes, the subcellular distribution of internalized HRP was analyzed. Confluent monolayers of L cells were treated with crude mouse interferon (1,000 U/ml) for 24 h before HRP was added. The cells were then homogenized, and the postnuclear supernatants were centrifuged in isopycnic sucrose density gradients. The distribution of the HRP internalized by interferon-treated and untreated cells paralleled the distribution of the lysosomal marker N-acetyl-p-glucosaminidase (Fig. 2).When L cells were treated for 24 h with increasing concentrations of crude mouse interferon, slight inhibition of HRP uptake was apparent at concentrations of 1 and 10 U/ml, and 50% inhibition was observed at 100 U/ml. At the highest dose tested (1,000 U/ml), HRP uptake was inhibited by 75% (Fig. 3). Similar doseresponse data were obtained when L cells were treated with a purified mouse interferon preparation (Fig. 3).HRP uptake was analyzed as a function of time after the addition of 1,000 U of interferon per ml to L cells. There was no detectable effect on HRP uptake at 4 h; however, by 8 h after the addition of the inhibitor, a 25% reduction was seen. By 14 h the rate of uptake had decreased to 1.3 ng/mg per min, a 50% reduction. The greatest inhibition (a decrease to 28% of control levels) was observed at 24 h (Fig. 4).Cells which had been treated with 1,000 U of interferon per ml for 24 h were th...

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mentioning

confidence: 99%

Interferon treatment inhibits pinocytosis.

Wilcox¹,

Whitaker-Dowling²,

Youngner³

et al. 1983

Mol. Cell. Biol.

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“…Both studies confirmed broad antiviral activity of 25HC in vitro against different classes of lipid-enveloped RNA and DNA viruses. This was subsequently reaffirmed by several independent studies (Arita et al 2013;Chen et al 2014;Mboko et al 2014), and the antiviral activity was additionally extended to nonenveloped viruses (Civra et al 2014). Table 1 summarizes the viruses whose susceptibility to 25HC's antiviral effects has been validated.…”

Section: Hc: Broad Antiviral Lipid Effectormentioning

confidence: 57%

Armand-Frappier Outstanding Student Award — The emerging role of 25-hydroxycholesterol in innate immunity

2015

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Abstract:The metabolic interplay between hosts and viruses plays a crucial role in determining the outcome of viral infection. Viruses reorchestrate the host's primary metabolic gene networks, including genes associated with mevalonate and isoprenoid synthesis, to acquire the necessary energy and structural components for their viral life cycles. Recent work has demonstrated that the interferon-mediated antiviral response suppresses the sterol pathway through production of a signalling molecule, 25-hydroxycholesterol (25HC). This oxysterol has been shown to exert multiple effects, both through incorporation into host cellular membranes as well as through transcriptional control. Herein, we summarize our current understanding of the multifunctional roles of 25HC in the mammalian innate antiviral response.Key words: 25-hydroxycholesterol, cholesterol-25-hydroxylase, metabolism, virus, immunity.Résumé : Les interactions métaboliques entre les hôtes et les virus jouent un rôle crucial qui déterminera l'issue de l'infection virale. Les virus réorganisent les réseaux de gènes métaboliques primaires de l'hôte, dont les gènes liés à la synthèse du mévalonate et des isoprénoïdes, afin d'acquérir l'énergie et les éléments structuraux néces-saires à leur cycle de vie. Des travaux récents ont démontré que la réponse antivirale activée par les interférons supprime la voie des stérols par la production d'une molécule de signalisation, le 25-hydroxycholestérol (25HC). On a révélé que cet oxystérol avait plus d'un effet, tant par son intégration dans les membranes de la cellule-hôte que par le contrôle de la transcription. Nous résumons ici notre conception actuelle des rôles multifonctionnels du 25HC dans la réponse antivirale innée chez les mammifères. [Traduit par la Rédaction] -clés : 25-hydroxycholestérol, cholestérol-25-hydroxylase, métabolisme, virus, immunité. Mots

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“…IFN inhibits the production of viral glycoproteins, thus affecting the membrane-associated steps of viral replication (Chatterjee et al, 1985). Alternatively, IFN may change the fluidity of membranes and thereby disrupt viral morphogenesis (Chatterjee et al, 1982;Pfeffer et al, 1981 ;Wang et al, 1981).…”

Section: Discussionmentioning

confidence: 99%

The influence of porcine recombinant interferon- 1 on pseudorabies virus infection of porcine nasal mucosa in vitro

Pol¹,

Broekhuysen-Davies²,

Wagenaar³

et al. 1991

Journal of General Virology

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To determine the effect of interferon (IFN) on the pathogenesis of pseudorabies virus (PRV), porcine nasal mucosal explants were first treated with recombinant porcine methionyl-IFN-atl and then infected with one of three strains of PRV. The stroma of treated mucosal explants were protected against infection with virulent PRV or PRV of intermediate virulence because the infection was restricted to the epithelial cells. In contrast, untreated mucosal explants were readily infected by virulent PRV or PRV of intermediate virulence; the infection spread from epithelial cells to stromal fibroblasts. Avirulent PRV infection was restricted to the epithelial cells of treated and untreated mucosal explants. IFN treatment limited the extent of all three PRV infections in the epithelial cells. Cultured porcine fibroblasts and porcine kidney cells were also treated with IFN and subsequently infected with PRV; infection was prevented in most porcine fibroblasts and the virus yield from porcine kidney cells was reduced. Budding of virulent PRV nucleocapsids through the inner nuclear membrane was observed more frequently in treated than in untreated mucosal explants and enveloped virus particles accumulated between the inner and outer nuclear membranes, indicating that the membrane-associated events of PRV replication had been affected. We conclude that IFN-at protects stromal fibroblasts against PRV infection and reduces virus replication in epithelial cells.

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Interferon inhibits Sendai virus-induced cell fusion: an effect on cell membrane fluidity.

Cited by 43 publications

References 30 publications

Interferon treatment inhibits pinocytosis.

Interferon treatment inhibits pinocytosis.

Armand-Frappier Outstanding Student Award — The emerging role of 25-hydroxycholesterol in innate immunity

The influence of porcine recombinant interferon- 1 on pseudorabies virus infection of porcine nasal mucosa in vitro

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