On the Control of Immediate Early ( ) mRNA Survival in Cells Infected with Herpes Simplex Virus

Fenwick, M. L.; Owen, S. A.

doi:10.1099/0022-1317-69-11-2869

Cited by 29 publications

(34 citation statements)

References 5 publications

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“…This suggestion was based on the observation that after mixed infection, HSV-I(F), which expresses stable IE mRNAs, stabilized the normally unstable IE mRNA of HSV-2(G) (Fenwick & Clark, 1982. It was observed later that the stability ofIE mRNA was determined by a gene or genes between 0.58 and 0-65 map units and that if the dominance of mRNA stability over strong shutoff seen in mixed infection also determined the phenotypes of intertypic recombinant viruses, then the specific hypothetical mRNA-stabilizing factor mapped in this region (Fenwick & Owen, 1988). However the present results show that the opposite is true: in recombinants 17G41 and 17(41-)G41 the strong shutoff of HSV-2(G) is dominant.…”

Section: Discussionmentioning

confidence: 99%

“…It is known that the half-lives of all mRNAs of HSV-I(KOS) (1 to 2 h) were considerably increased by a mutation in the vhs gene, UL41 (Read & Frenkel, 1983;Kwong & Frenkel, 1987;Oroskar & Read, 1987 and the exceptional instability of the IE mRNA of HSV-2(G) in the presence of CX (half-life of about 15 min) may reflect the action of a strong shutoff protein on mRNA unprotected by ribosomes. The RNA accumulated in stable form after removal of CX or during normal infection (Fenwick & Owen, 1988). The apparent discrimination of the shutoff mechanism between host and viral protein synthesis may be explained by the hypothesis that the shutoff activity is short-lived (Fenwick & Owen, 1988) and degradation of mRNA induced by UL41 is more than counterbalanced by the increasing rate of transcription of viral mRNA while that of cellular mRNA is steady or declining.…”

Section: Discussionmentioning

confidence: 99%

“…The RNA accumulated in stable form after removal of CX or during normal infection (Fenwick & Owen, 1988). The apparent discrimination of the shutoff mechanism between host and viral protein synthesis may be explained by the hypothesis that the shutoff activity is short-lived (Fenwick & Owen, 1988) and degradation of mRNA induced by UL41 is more than counterbalanced by the increasing rate of transcription of viral mRNA while that of cellular mRNA is steady or declining.…”

Section: Discussionmentioning

confidence: 99%

“…HSV-I(17 +) causes only slight inhibition, and its IE mRNA accumulates in the presence of cycloheximide (CX) added at the time of infection and is translated on removal of the inhibitor. In contrast, HSV-2(G) shuts off host synthesis strongly; also its IE mRNA is very unstable and does not accumulate unless protein synthesis is allowed (Fenwick & Clark, 1983;Fenwick & Owen, 1988). To investigate the functions of gene UL41 and in particular the question of whether it alone determines both phenotypes, we have isolated the analogous gene from HSV-2(G) and inserted it into the non-essential thymidine kinase (TK) gene of HSV-I(17+).…”

Section: Introductionmentioning

confidence: 99%

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Transfer of UL41, the gene controlling virion-associated host cell shutoff, between different strains of herpes simplex virus

Fenwick

Everett²

1990

Journal of General Virology

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Transfer of UL41, the gene controlling virion-associated host cell shutoff, between different strains of herpes simplex virus

Fenwick

Everett²

1990

Journal of General Virology

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“…vhs, a 489-amino-acid phosphoprotein that, like VP16, exists as a preformed viral structural component, disables host protein synthesis and triggers mRNA degradation following infection (13,24,25,35,40,43,47,52). vhs is not required for HSV-1 propagation in tissue culture, although in its absence, the expression of viral proteins is altered during an infection and there is a significant reduction in virus yield (39,40).…”

mentioning

confidence: 99%

A Single Amino Acid Substitution in Herpes Simplex Virus Type 1 VP16 Inhibits Binding to the Virion Host Shutoff Protein and Is Incompatible with Virus Growth

Knez

Bilan

Capone

2003

J Virol

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In addition to its well-established role in the activation of herpes simplex virus immediate-early gene transcription, VP16 interacts with and downregulates the function of the virion host shutoff protein (vhs), thereby attenuating vhs-mediated destruction of viral mRNAs and translational arrest at late times of infection. We have carried out two-hybrid analysis in vivo and protein-protein interaction assays in vitro to identify determinants in VP16 necessary for interaction with vhs. The minimal amino-terminal subfragment of VP16 capable of binding to vhs encompassed residues 1 to 345. Alteration of a single leucine at position 344 to alanine (L344A) in the context of the amino-terminal fragment of VP16 containing residues 1 to 404 was sufficient to abolish interaction with vhs in vitro and in vivo. Leu344 could be replaced with hydrophobic amino acids (Ile, Phe, Met, or Val) but not by Asn, Lys, or Pro, indicating that hydrophobicity is an important property of binding to vhs. VP16 harboring a loss-of-function mutation at L344 was not compromised in its ability to interact with host cell factor (HCF-1) or to activate transcription of viral immediate-early genes in transient-transfection assays. Virus complementation assays using the VP16-null virus 8MA and the VP16/vhs double-mutant virus 8MA⌬Sma showed that VP16(L344A) was able to complement the growth of 8MA⌬Sma but not 8MA. Thus, a single point mutation in VP16 uncouples binding to vhs from other functions of VP16 required for virus growth and indicates that direct physical association between VP16 and vhs is necessary to sustain a productive infection.Herpes simplex virus type 1 (HSV-1) is a large, enveloped DNA virus whose genome encodes some 80 genes. These genes fall into three broad kinetic classes, depending on their order of appearance during a lytic infection: immediate early (IE or ␣), early (E or ␤), and late (L or ␥). Members of each class are coordinately and temporally regulated in a cascade fashion, primarily at the transcriptional level, by interactive networks that involve both virus and host factors. HSV-1 is noteworthy in that several important viral regulatory proteins exist as preformed structural components of the virion. These factors are delivered into the host cell by the infecting virus particle and are thus poised to affect the earliest events of viral infection and initiation of replication (reviewed in reference 41). The most prominent of these is the viral transactivator VP16, an abundant 490-amino-acid phosphoprotein contained in the viral tegument, an amorphous protein layer present between the viral capsid and envelope (5). VP16 possesses a potent C-terminal transactivation domain and triggers the lytic cycle by initiating IE gene expression via conserved cis-acting TAATGARAT elements present in the promoter regions of all the IE genes (2, 33, 38, 42, 51). VP16 on its own has only weak DNA binding activity, and efficient recruitment to promoter target sites relies on the assembly of a multicomponent protein/DNA binding transc...

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Herpes simplex virus VP16 rescues viral mRNA from destruction by the virion host shutoff function.

et al. 1996

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Herpes simplex virus (HSV) virions contain two regulatory proteins that facilitate the onset of the lytic cycle: VP16 activates transcription of the viral immediate‐early genes, and vhs triggers shutoff of host protein synthesis and accelerated turnover of cellular and viral mRNAs. VP16 and vhs form a complex in infected cells, raising the possibility of a regulatory link between them. Here we show that viral protein synthesis and mRNA levels undergo a severe decline at intermediate times after infection with a VP16 null mutant, culminating in virtually complete translational arrest. This phenotype was rescued by a transcriptionally incompetent derivative of VP16 that retains vhs binding activity, and was eliminated by inactivating the vhs gene. These results indicate that VP16 dampens vhs activity, allowing HSV mRNAs to persist in infected cells. Further evidence supporting this hypothesis came from the demonstration that a stably transfected cell line expressing VP16 was resistant to host shutoff induced by superinfecting HSV virions. Thus, in addition to its well known function as a transcriptional activator, VP16 stimulates viral gene expression at a post‐transcriptional level, by sparing viral mRNAs from degradation by one of the virus‐induced host shutoff mechanisms.

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On the Control of Immediate Early ( ) mRNA Survival in Cells Infected with Herpes Simplex Virus

Cited by 29 publications

References 5 publications

Transfer of UL41, the gene controlling virion-associated host cell shutoff, between different strains of herpes simplex virus

Transfer of UL41, the gene controlling virion-associated host cell shutoff, between different strains of herpes simplex virus

A Single Amino Acid Substitution in Herpes Simplex Virus Type 1 VP16 Inhibits Binding to the Virion Host Shutoff Protein and Is Incompatible with Virus Growth

Herpes simplex virus VP16 rescues viral mRNA from destruction by the virion host shutoff function.

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