Control of Influenza Virus Gene Expression: Quantitative Analysis of Each Viral RNA Species in Infected Cells

Hatada, Eriko; Hasegawa, Masakazu; Mukaigawa, Jun; Shimizu, Kazufumi; Fukuda, Ryūji

doi:10.1093/oxfordjournals.jbchem.a122702

Cited by 105 publications

(115 citation statements)

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“…The dependence of IFV virus export on the CRM1 pathway is well established and the TAP pathway has also been shown to be involved in IFV export [31]. In addition, several studies indicate specific inhibition of late viral gene expression after UV irradiation, LB, actinomycin D or DRB treatment [1,12,21,22,27]. These studies reported that the drugs DRB and LB, which were added at the beginning of the infection, did not inhibit viral mRNA synthesis completely and that viral transcripts were retained in the nucleus, consistent with our microscopy results.…”

Section: Discussionmentioning

confidence: 99%

Influenza infection modulates vesicular trafficking and induces Golgi complex disruption

et al. 2016

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Influenza A virus (IFV) replicates its genome in the nucleus of infected cells and uses the cellular protein transport system for genome trafficking from the nucleus to the plasma membrane. However, many details of the mechanism of this process, and its relationship to subsequent cytoplasmic virus trafficking, have not been elucidated. We examined the effect of nuclear transport inhibitors Leptomycin B (LB), 5,6 dichloro-1-b-D-ribofuranosyl-benzimidazole (DRB), the vesicular transport inhibitor Brefeldin A (BFA), the caspase inhibitor ZWEHD, and microtubule inhibitor Nocodazole (NOC) on virus replication and intracellular trafficking of viral nucleoprotein (NP) from the nucleus to the ER and Golgi. Also, we carried out complementary studies to determine the effect of IFV on intracellular membranes. Inhibition of the CRM1 and TAP-P15 nuclear transport pathways by DRB and LB blocked completely the export of virus. Inhibition of vesicular trafficking by BFA, NOC, and ZWEHD also affected influenza infection. Interestingly, IFV infection induced fragmentation of the Golgi complex resulting in diffuse distribution of large and small vesicles throughout the cytoplasm. Live-cell microscopy revealed expansion of Golgi localization signals indicating progressive dispersion of Golgi positive structures, resulting in the disassembly of the Golgi ribbon structure. Other vesicular components (Rab1b, ARF1 and GBF1) were also found to be required for IFV infection. Furthermore, the exact step at which IFV infection disrupts vesicle trafficking was identified as the ER-Golgi intermediate compartment. These findings suggest that IFV NP is trafficked from the nucleus via the CRM1 and TAP pathways. IFV modulates vesicular trafficking inducing disruption of the Golgi complex. These studies provide insight on the ways in which IFV affects intracellular trafficking of different host proteins and will facilitate identification of useful pharmaceutical targets to abrogate virus replication.

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Section: Discussionmentioning

confidence: 99%

Influenza infection modulates vesicular trafficking and induces Golgi complex disruption

et al. 2016

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“…The resulting RNA was extracted again with phenol-chloroform. A quantitative hybridization system was employed to measure the amount of the three types of virus-specific RNA (mRNA, cRNA and vRNA) for each of the eight genome segments as reported elsewhere (Hatada et al, 1989), in which RNA probes intensely labelled with 32p were used in a molar excess sufficient to overpower complementary RNAs present in the viral RNA samples. The probes for mRNA and cRNA were obtained by transcribing SP 6 recombinant DNAs, which gave the intact 5' end sequences of vRNAs.…”

Section: Methodsmentioning

confidence: 99%

“…Several studies have been carried out to reveal the relationship between the synthesis of viral RNAs and proteins (Lamb & Choppin, 1976;Hay et al, 1977b;Inglis & Mahy, 1979;Barrett et al, 1979;Smith & Hay, 1982;Enami et al, 1985 ;Shapiro et al, 1987;Hatada et al, 1989). In MDCK cells infected with A/Udorn/72 (H3N2) virus, the synthesis of virus-specific RNAs proceeds as follows (Hatada et al, 1989).…”

Section: Introductionmentioning

confidence: 99%

“…In MDCK cells infected with A/Udorn/72 (H3N2) virus, the synthesis of virus-specific RNAs proceeds as follows (Hatada et al, 1989). During primary transcription at early times of infection, considerable amounts of mRNA are produced from the non-structural protein (NS), nucleoprotein (NP) and the three polymerase genes (early proteins), but very low amounts from the haemagglutinin (HA), neuraminidase (NA) and matrix protein (M) genes (late proteins).…”

Section: Introductionmentioning

confidence: 99%

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Involvement of the influenza A virus PB2 protein in the regulation of viral gene expression

Mukaigawa

Hatada

Fukuda

et al. 1991

Journal of General Virology

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To determine the function(s) of the PB2 protein of influenza A virus, six temperature-sensitive (ts) mutants of A/Udorn/72 (H3N2) virus, each carrying a ts mutation in the PB2 gene, were analysed for virus RNA and protein synthesis. One of the mutants, ICRC27, exhibited unique phenotypes and was characterized in detail. At the non-permissive temperature, 40 °C, the accumulation of mRNA for each genome segment was reduced severely, leading to delayed and reduced synthesis of viral proteins, complementary and viral RNAs (cRNAs and vRNAs). At the permissive temperature, 34 °C, the mutant virus produced severalfold greater concentrations of both mRNAs and cRNAs of PB2, PB1 and PA segments than wild-type virus. The synthesis of the three polymerase proteins and the induction of RNA polymerase activity were also greatly increased. By contrast, the expression of the haemagglutinin (HA) gene was severely suppressed. The over-production of the polymerase mRNAs was not observed during primary transcription, i.e. in the presence of cycloheximide. The ts ÷ revertants oflCRC27 did not exhibit the ts defects and also lost most of the non-ts phenotypes at 34 °C. These observations indicate that the PB2 protein participates not only in the synthesis of viral RNAs, but also in the regulation of viral gene expression, i.e. in the downregulation of the three polymerase genes and the upregulation of the HA gene during secondary transcription.

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“…Consequently, it was concluded that there must be some form of segment specificity in genome packaging (Laver & Downie, 1976;Nakajima & Sugiura, 1977). Further support was lent to the segment-specific packaging model by the observation that segments were present at equimolar levels in virions (Hatada et al, 1989;McGeoch et al, 1976) even when their ratios in infected cells differed (Bergmann & Muster, 1995;Smith & Hay, 1982), suggesting that some form of selection process was operating.…”

Section: Genome Segmentation: a Mixed Blessingmentioning

confidence: 99%

Genome packaging in influenza A virus

Hutchinson

Kirchbach

Gog

et al. 2009

Journal of General Virology

256

279

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Control of Influenza Virus Gene Expression: Quantitative Analysis of Each Viral RNA Species in Infected Cells

Cited by 105 publications

References 0 publications

Influenza infection modulates vesicular trafficking and induces Golgi complex disruption

Influenza infection modulates vesicular trafficking and induces Golgi complex disruption

Involvement of the influenza A virus PB2 protein in the regulation of viral gene expression

Genome packaging in influenza A virus

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