Dissecting Herpes Simplex Virus 1-Induced Host Shutoff at the RNA Level

Friedel, Caroline C.; Whisnant, Adam W.; Djaković, Lara; Rutkowski, A.; Friedl, Marie-Sophie; Kluge, Michael; Williamson, James C; Sai, Somesh; Vidal, Ramón; Sauer, Sascha; Hennig, Thomas; Grothey, Arnhild; Milic, Andrea; Prusty, Bhupesh K.; Lehner, Paul J.; Matheson, Nicholas J; Erhard, Florian; Dölken, Lars

doi:10.1128/jvi.01399-20

Cited by 36 publications

(56 citation statements)

References 86 publications

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“…We found that within 4h of HSV-1 infection of human cells there are dramatic changes to the host cell mRNA transcriptional program, with hundreds of genes losing Pol II occupancy and hundreds of others gaining Pol II. This is largely consistent with the transcriptional reprogramming observed in prior studies that also studied the effect of HSV-1 infection on host cell transcription in human cells looking at nascent mRNA production via PRO-seq or 4SU-seq rather than using Pol II ChIP-seq [10,11,13,39,40]. The effect of HSV-1 infection on Pol II occupancy in human cells is significantly different from that seen in mouse cells where only the reduction of Pol II occupancy was observed after 4h of infection with little to no activation [12], suggesting that the activation of Pol II transcription is a signature specific to the host species.…”

Section: Discussionsupporting

confidence: 86%

The herpes simplex virus 1 protein ICP4 acts as both an activator and repressor of host genome transcription during infection

Rivas

Goodrich

Kugel

2021

Preprint

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Infection by Herpes simplex virus 1 (HSV-1) impacts nearly all steps of gene expression in the host cell. The regulatory mechanisms by which this occurs, and the interplay between host and viral factors, have yet to be fully elucidated. Here we investigated how the occupancy of RNA polymerase II (Pol II) on the host genome changes during HSV-1 infection and is impacted by the viral immediate early protein ICP4. Pol II ChIP-seq experiments revealed a reduction of Pol II occupancy across the bodies of hundreds of host genes that was dependent upon ICP4. Concomitantly, Pol II levels increased across the bodies of several hundred genes, the majority of which also depended on ICP4 for activation. Our data suggest ICP4 regulates repression of Pol II at host genes by inhibiting recruitment of Pol II, while it regulates activation by promoting release of Pol II from promoter proximal pausing into productive elongation. Consistent with this, relative levels of the pausing factors NELF-A and Spt5 were reduced on an HSV-1 activated gene in an ICP4 dependent manner. Exogenous expression of ICP4 revealed that ICP4 can activate, but not repress, transcription of some genes in the absence of infection in a manner that correlates with the chromatin state of the gene. Together our data support the model that ICP4 decreases promoter proximal pausing on host genes activated by infection, and ICP4 is necessary, but not sufficient, to repress transcription from host genes during viral infection.

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Section: Discussionsupporting

confidence: 86%

The herpes simplex virus 1 protein ICP4 acts as both an activator and repressor of host genome transcription during infection

Rivas

Goodrich

Kugel

2021

Preprint

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“…In a recent study, we observed that the upregulation of the cellular protein Tripartite-motif 43 (TRIM43) upon HSV-1 infection is dependent on the embryonic transcription factor DUX4 7 , which was recently confirmed by Friedel et al 8 . DUX4 is a germline transcription factor exclusively expressed from the 4-cell to the 8-cell state, a short phase during human embryonic development [9][10][11] .…”

Section: Introductionsupporting

confidence: 56%

Herpesviral induction of germline transcription factor DUX4 is critical for viral gene expression

Walter

Franke

Drayman

et al. 2021

Preprint

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DUX4 is a transcription factor and a master regulator of embryonic genome activation (EGA). During early embryogenesis, EGA is crucial for maternal to zygotic transition at the 8-cell stage in order to overcome silencing of genes and enable transcription from the zygotic genome. In adult somatic cells, DUX4 expression is largely silenced. Activation is likely pathogenic, and in adult muscle cells causes genetic disorder Facioscapulohumeral Muscular Dystrophy (FSHD). We identified activation of DUX4 expression upon lytic replication of the herpesviruses HSV-1, HCMV, EBV and KSHV, but not of adenoviruses, negative strand RNA viruses or positive strand RNA viruses. We demonstrate by RNA-Seq analysis that DUX4 expression upon herpesviral replication leads to the induction of hundreds of DUX4 target genes including germline-specific retroelements as well as several members of the TRIM, PRAMEF and ZSCAN protein families. Moreover, we show that DUX4 expression is a direct consequence of herpesviral infection. DUX4 can be stimulated by overexpression of HSV-1 immediate early proteins, indicating active induction of EGA genes by herpesviral infection. We further show that DUX4 expression is critical for driving HSV-1 gene expression. Our results show that viruses from alpha-, beta- and gamma-herpesvirus subfamilies induce DUX4 expression and downstream germline-specific genes and retroelements. We hypothesize that herpesviruses induce DUX4 expression in order to induce an early embryonic-like transcriptional program that prevents epigenetic silencing of the viral genome and facilitates herpesviral gene expression.

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“…While recent studies have identified many interesting findings from total RNA analysis [131][132][133][134][135], general conclusions at the level of transcription are complicated by the varying technical methods and biological contexts utilized. Interestingly, nuclease activity of VHS globally reduced Pol II transcription of host genes, as was observed before with the SOX nuclease from murine gamma-herpesvirus 68 (MHV68) [111,136]. A proper discussion of host mRNA accumulation, its translation, and resulting outcomes on infection, particularly regarding innate immunity, is outside the scope of this review.…”

Section: Broader Network and Future Considerationsmentioning

confidence: 71%

“…Such techniques include those using chemical labeling (e.g., 4sU-Seq), long-read sequencing, or minimally normalization of polyadenylated RNA to chromatin-associated rather than total/total nuclear RNA. Chromatin-associated RNA closely matches nascent transcriptomes determined by chemical labeling in HSV infection [111], and is currently the most cost-effective and procedurally simple approach to differentiate co-from post-transcriptional events directly compatible with established HSV infection protocols for total RNA.…”

Section: Rna Processing In Splicing and Terminationmentioning

confidence: 87%

“…While microarray studies indicated the seeming induction of several host genes [128][129][130], particularly antiviral responses, viral and cellular profiles induced are highly variable between individual cells and depend on various factors that include virus dose, virus stock quality, viral genetic variability, the status of the cell and cell type tested. Notably, RNA-Seq data has to be carefully analyzed to avoid misinterpretations as many transcripts are affected by termination failure and, in turn, are atypically spliced, might extend into downstream genes, and, more importantly, fail to get exported to the cytoplasm [81,82,111]. The post-transcriptional stability and, thereby, viral and cellular RNA levels are regulated by the nuclease activity of the aptly named virion host shutoff (VHS) protein, further complicating conclusions of transcriptional regulation from the level of total, cytoplasmic, or polyadenylated RNA.…”

Section: Broader Network and Future Considerationsmentioning

confidence: 99%

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A Review of the Multipronged Attack of Herpes Simplex Virus 1 on the Host Transcriptional Machinery

Hennig

Djaković

Dölken

et al. 2021

Viruses

Self Cite

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During lytic infection, herpes simplex virus (HSV) 1 induces a rapid shutoff of host RNA synthesis while redirecting transcriptional machinery to viral genes. In addition to being a major human pathogen, there is burgeoning clinical interest in HSV as a vector in gene delivery and oncolytic therapies, necessitating research into transcriptional control. This review summarizes the array of impacts that HSV has on RNA Polymerase (Pol) II, which transcribes all mRNA in infected cells. We discuss alterations in Pol II holoenzymes, post-translational modifications, and how viral proteins regulate specific activities such as promoter-proximal pausing, splicing, histone repositioning, and termination with respect to host genes. Recent technological innovations that have reshaped our understanding of previous observations are summarized in detail, along with specific research directions and technical considerations for future studies.

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Dissecting Herpes Simplex Virus 1-Induced Host Shutoff at the RNA Level

Cited by 36 publications

References 86 publications

The herpes simplex virus 1 protein ICP4 acts as both an activator and repressor of host genome transcription during infection

The herpes simplex virus 1 protein ICP4 acts as both an activator and repressor of host genome transcription during infection

Herpesviral induction of germline transcription factor DUX4 is critical for viral gene expression

A Review of the Multipronged Attack of Herpes Simplex Virus 1 on the Host Transcriptional Machinery

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