Differential efficacies of human type I and type II interferons as antiviral and antiproliferative agents.

Rubin, Berish Y.; Gupta, Saloni

doi:10.1073/pnas.77.10.5928

Cited by 244 publications

(82 citation statements)

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“…2 and 3), cultured skin fibroblasts from newborn or adult donors, and some transformed or tumor cell lines (data not shown). Human fibroblast proteins with apparent molecular sizes of about 80,000 Da that are strongly induced by IFN-a but not detectably induced by IFN-y have previously been described by two other groups (7,11). It remains to be determined whether one of these proteins and the 2C12-cross-reacting protein are identical.…”

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confidence: 99%

“…They induce in responsive cells the synthesis of several proteins that are not detected or do exist at much lower concentrations in untreated cells. Induced proteins in mouse and human cells have been widely studied (1,5,7,10,11; for a review, see reference 6), but most of them are still poorly characterized. Also, little is known about the functional, structural, and evolutionary relationships of distinct proteins induced in cells of different species.…”

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confidence: 99%

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Interferon-induced human protein with homology to protein Mx of influenza virus-resistant mice.

Staeheli¹,

Haller²

1985

Mol. Cell. Biol.

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Polyclonal and monoclonal antibodies with specificity for protein Mx (a karyophilic 75,000-dalton protein induced by interferon [IFN] in mouse cells carrying the influenza virus resistance allele Mx+) detected an IFN-induced 80,000-dalton protein in peripheral blood lymphocytes and in fibroblasts of healthy human donors. The human protein, like protein Mx, was induced by IFN-a but not by IFN-'y. Unlike the mouse protein, it was predominantly localized in the cell cytoplasm.

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confidence: 99%

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confidence: 99%

Interferon-induced human protein with homology to protein Mx of influenza virus-resistant mice.

Staeheli¹,

Haller²

1985

Mol. Cell. Biol.

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“…CTS-51 was isolated in the process of the immune interferon production. However it does not show any antiviral activity at all, and the cytotoxic activity of CTS-51 is preserved even after the acid treatment at pH 2.0 for 24 hr, where IFN-y is known to be inactivated (Rubin and Gupta 1980). These observations seem to deny the possibilities that CTS-51 is one of the immune interferons nor that the cytotoxic activity of IFN-y preparations may be exerted by this cytotoxic substance contaminated in them.…”

Section: Discussionmentioning

confidence: 37%

“…Some of these factors, such as, for example, interferons and interleukin-2, are revealed to have a property to potentiate the cytotoxic activities of several cellular immunological systems, such as, for example, natural killer cell system or MLC derived cell mediated cytotoxicity system (Heron et al 1976(Heron et al , 1979Marx 1983). On the other hand, several other cytokines have been reported to have a property directly cytotoxic to the target cells in vitro, which include lymphotoxins (Evans 1982), tumor necrosis factors (williamson et al 1983), natural killer cytotoxic factors (Bonavida et al 1982) and immune interferons (Rubin and Gupta 1980).…”

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A cytotoxic substance (CTS-51) produced by human buffy coat cultures stimulated by Staphylococcal enterotoxin B: Further characterizations and combined action with interferon.

Hirai

Hattori

Georgiades³

et al. 1986

Tohoku J. Exp. Med.

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A recently recognized unique cytotoxic substance, CTS 51, was tested for the heat or acid stability, trypsin digestion and dialysis. Moreover, influences of elevated incubation temperatures or serum concentrations of medium on the cytotoxic activity of CTS-51, and the combination effects of CTS-51 and human leucocyte interferon (TuIFN-a (Le)) were investigated. The cytotoxic activity of CTS-51, which is promoted by a small molecule easily passable the dialysis membrane, was found to be very stable to heat (even at 100°C for 30 min) or acid (pH 2.0 for 24 hr at 4°C) treatments. The treatment with 0.75° trypsin for lhr did not diminish the CTS 51 activity. The susceptibility of Daudi lymphoma cells to the antiproliferative action of HuIFN-a (Le) was further potentiated by treating the cells with CTS-51 for 16 hr. On the other hand, the CTS-51 activity which was revealed to be prescribed by its concentration in the medium, was not potentiated at 39°C when compared to that at 37°C in contrast to HuIFN-a (Le) action, and was reduced according to the increase of the fetal calf serum concentration in the medium.cytokine ; interferon ; cytotoxicity It is generally known that lymphocytes or monocytes, when activated by the antigen-or mitogen-stimulation, release a mixture of several biologically active soluble factors, with various molecular sizes, which are usually called lymphokines or monokines, generally called "cytokines" as a whole (Evans 1982). It has been argued, from several quarters (Evans 1982;Ransom and Evans 1982;

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“…The lack of anti-adenovirus action of rlFN-~ suggests that the effect of rlFN-y depends on some mechanism(s) not shared by rlFN-a. The possibility of rlFN-y acting by a different antiviral mechanism was previously discussed by Rubin & Gupta (1980), who showed that vaccinia virus and reovirus were sensitive to IFN-y but not to IFN-a. Weil et al (1983) have shown the synthesis after rIFN-7 treatment of at least eight polypeptides not induced by rIFN-e. Antiviral states induced by IFN-cc/fl and IFN-y have been shown to be regulated with different kinetics, for both induction and extinction (Ramamurthy & Fleischmann, 1986).…”

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Recombinant Human Interferon- Inhibits Adenovirus Multiplication without Modifying Viral Penetration

Mistchenko

Díez

Falcoff

1987

Journal of General Virology

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SUMMARYWe have recently reported that adenovirus replication is inhibited by human recombinant interferon-y, but not by recombinant interferon-cq in a dose-dependent manner. The aim of this study was to determine whether the antiviral effect of recombinant interferon-~ could be linked to interferon-induced alteration at the membrane level, inhibiting either adenovirus penetration of or release from WISH cells. Adsorption and penetration were investigated with an 12SI-labelled adenovirus binding assay. To test defective virus release, the presence of newly synthesized virus proteins in the cytoplasmic and nuclear compartments was investigated. Binding studies showed that interferons-7 and -a did not modify adenovirus attachment and penetration. Interferon-y but not interferon-a inhibited hexon protein synthesis in the cytosol as well as its accumulation in the nuclear compartment. The synthesis of polypeptides III, IV and VI was also inhibited. In cells infected before interferon-7 treatment, its addition could be delayed up to 2 h after the infection to produce an inhibition of virus yield greater than 1 log10 unit (90~ inhibition). We conclude that interferon-y acts on an intracellular step before or at adenovirus protein synthesis, probably through a mechanism not shared with interferon-a.

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Differential efficacies of human type I and type II interferons as antiviral and antiproliferative agents.

Cited by 244 publications

References 36 publications

Interferon-induced human protein with homology to protein Mx of influenza virus-resistant mice.

Interferon-induced human protein with homology to protein Mx of influenza virus-resistant mice.

A cytotoxic substance (CTS-51) produced by human buffy coat cultures stimulated by Staphylococcal enterotoxin B: Further characterizations and combined action with interferon.

Recombinant Human Interferon- Inhibits Adenovirus Multiplication without Modifying Viral Penetration

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