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Literature DB >> 10982346

Herpes simplex virus 1 open reading frames O and P are not necessary for establishment of latent infection in mice.

Abstract

Open reading frame (ORF) O and ORF P partially overlap and are located antisense to the gamma(1)34.5 gene within the domain transcribed during latency. In wild-type virus-infected cells, ORF O and ORF P are completely repressed during productive infection by ICP4, the major viral transcriptional activator/repressor. In cells infected with a mutant in which ORF P was derepressed there was a significant delay in the appearance of the viral alpha-regulatory proteins ICP0 and ICP22. The ORF O protein binds to and inhibits ICP4 binding to its cognate DNA site in vitro. These characteristics suggested a role for ORF O and ORF P in the establishment of latency. To test this hypothesis, two recombinant viruses were constructed. In the first, R7538(P-/O-), the ORF P initiator methionine codon, which also serves as the initiator methionine codon for ORF O, was replaced and a diagnostic restriction endonuclease was introduced upstream. In the second, R7543(P-/O-)R, the mutations were repaired to restore the wild-type virus sequences. We report the following. (i) The R7538(P-/O-) mutant failed to express ORF O and ORF P proteins but expressed a wild-type gamma(1)34.5 protein. (ii) R7538(P-/O-) yields were similar to that of the wild type following infection of cell culture or following infection of mice by intracerebral or ocular routes. (iii) R7538(P-/O-) virus reactivated from latency following explanation and cocultivation of murine trigeminal ganglia with Vero cells at a frequency similar to that of the wild type, herpes simplex virus 1(F). (iv) The amount of latent R7538(P-/O-) virus as assayed by quantitative PCR is eightfold less than that of the repair virus. The repaired virus could not be differentiated from the wild-type parent in any of the assays done in this study. We conclude that ORF O and ORF P are not essential for the establishment of latency in mice but may play a role in determining the quantity of latent virus maintained in sensory neurons.

Entities: Chemical Disease Gene Species

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Year: 2000 PMID： 10982346 PMCID： PMC102098 DOI： 10.1128/jvi.74.19.9019-9027.2000

Source DB: PubMed Journal: J Virol ISSN： 0022-538X Impact factor: 5.103

60 in total

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Journal: J Virol Date: 1996-04 Impact factor: 5.103

2. Phenotypic properties of herpes simplex virus 1 containing a derepressed open reading frame P gene.

Authors: M Lagunoff; G Randall; B Roizman
Journal: J Virol Date: 1996-03 Impact factor: 5.103

3. Regulation of herpesvirus macromolecular synthesis. I. Cascade regulation of the synthesis of three groups of viral proteins.

Authors: R W Honess; B Roizman
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4. The regulation of synthesis and properties of the protein product of open reading frame P of the herpes simplex virus 1 genome.

Authors: M Lagunoff; B Roizman
Journal: J Virol Date: 1995-06 Impact factor: 5.103

5. Quantification of transcripts from the ICP4 and thymidine kinase genes in mouse ganglia latently infected with herpes simplex virus.

Authors: M F Kramer; D M Coen
Journal: J Virol Date: 1995-03 Impact factor: 5.103

6. Repression of the herpes simplex virus 1 alpha 4 gene by its gene product (ICP4) within the context of the viral genome is conditioned by the distance and stereoaxial alignment of the ICP4 DNA binding site relative to the TATA box.

Authors: R Leopardi; N Michael; B Roizman
Journal: J Virol Date: 1995-05 Impact factor: 5.103

7. High-dose ocular infection with a herpes simplex virus type 1 ICP34.5 deletion mutant produces no corneal disease or neurovirulence yet results in wild-type levels of spontaneous reactivation.

Authors: G C Perng; H Ghiasi; S M Slanina; A B Nesburn; S L Wechsler
Journal: J Virol Date: 1996-05 Impact factor: 5.103

8. The role of ICP4 repressor activity in temporal expression of the IE-3 and latency-associated transcript promoters during HSV-1 infection.

Authors: R Rivera-Gonzalez; A N Imbalzano; B Gu; N A Deluca
Journal: Virology Date: 1994-08-01 Impact factor: 3.616

9. An avirulent ICP34.5 deletion mutant of herpes simplex virus type 1 is capable of in vivo spontaneous reactivation.

Authors: G C Perng; R L Thompson; N M Sawtell; W E Taylor; S M Slanina; H Ghiasi; R Kaiwar; A B Nesburn; S L Wechsler
Journal: J Virol Date: 1995-05 Impact factor: 5.103

10. Replication, establishment of latent infection, expression of the latency-associated transcripts and explant reactivation of herpes simplex virus type 1 gamma 34.5 mutants in a mouse eye model.

Authors: J G Spivack; M U Fareed; T Valyi-Nagy; T C Nash; J S O'Keefe; R M Gesser; E A McKie; A R MacLean; N W Fraser; S M Brown
Journal: J Gen Virol Date: 1995-02 Impact factor: 3.891

11 in total

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Authors: Shun-Hua Chen; Lily Yeh Lee; David A Garber; Priscilla A Schaffer; David M Knipe; Donald M Coen
Journal: J Virol Date: 2002-05 Impact factor: 5.103

Review 2. Peculiarities of herpes simplex virus (HSV) transcription: an overview.

Authors: Július Rajcáni; Vojvodová Andrea; Rezuchová Ingeborg
Journal: Virus Genes Date: 2004-04 Impact factor: 2.332

Review 3. Herpes simplex virus-1 and varicella-zoster virus latency in ganglia.

Authors: Bradley M Mitchell; David C Bloom; Randall J Cohrs; Donald H Gilden; Peter G E Kennedy
Journal: J Neurovirol Date: 2003-04 Impact factor: 2.643

4. Characterization of herpes simplex virus 2 primary microRNA Transcript regulation.

Authors: Shuang Tang; Marta Bosch-Marce; Amita Patel; Todd P Margolis; Philip R Krause
Journal: J Virol Date: 2015-02-11 Impact factor: 5.103

5. The herpes simplex virus type 1 BgKL variant, unlike the BgOL variant, shows a higher association with orolabial infection than with infections at other sites, supporting the variant-dispersion-replacement hypothesis.

Authors: Shigeru Ozawa; Hiroyuki Eda; Yasuyuki Ishii; Fumihiko Ban; Toshiyuki Funabashi; Seiichiro Hata; Kozaburo Hayashi; Hiroki Iga; Takao Ikushima; Hiroaki Ishiko; Tomoo Itagaki; Rinji Kawana; Shunsaku Kobayashi; Takeo Ogino; Tsuyoshi Sekizawa; Yoshikazu Shimomura; Hiroshi Shiota; Ryoichi Mori; Takashi Nakakita; Yoshio Numazaki; Yoshikatsu Ozaki; Shigeru Yamamoto; Kamesaburo Yoshino; Kazuo Yanagi
Journal: J Clin Microbiol Date: 2007-05-02 Impact factor: 5.948