Cloning, sequencing, and functional analysis of oriL, a herpes simplex virus type 1 origin of DNA synthesis.

SUMMARYAlthough all herpesviruses are similar in their temporal regulation of gene expression, the organization of the immediate early (IE) genes varies markedly between the different members of the group. Most of the IE transcripts of human cytomegalovirus originate from a restricted region within the long unique segment of its linear dsDNA genome of 235 kb. One of the predominant transcripts from the IE region is a 5 kb RNA. Northern blot analyses revealed that this class of RNA is continuously present in infected cells. It was detected at high levels in IE and late RNA preparations, and in low amounts in early RNA preparations. It was not confined to the poly(A) + fraction upon oligo(dT) selection, but also appeared in similar amounts in poly(A)-fractions. Fine mapping of this transcript was done by nuclease protection and primer extension. The RNA appeared to be unspliced, and no signals such as TATA or CCAAT, known to be important elements in eukaryotic RNA polymerase II promoters, were found close to the 5' end. Sequence analysis revealed multiple stop codons throughout the AT-rich potential coding region. Since no splicing was found to occur, the largest protein deduced from the DNA sequence would be of not more than 12000 Mr. However, a computer program designed to detect protein-coding DNA sequences by codon usage did not reveal significant evidence for a protein encoded in this region. Therefore this RNA is likely to represent an unprecedented case of a large non-coding transcript present in cells that are lytically infected by an animal virus.

Section: Dna Sequence Analysismentioning

confidence: 99%

Abundant 5 kb RNA of Human Cytomegalovirus without a Major Translational Reading Frame

Plachter

Traupe²,

Albrecht³

et al. 1988

“…1 ; for review, see Roizman, 1979). Origins of DNA replication have been located in two distinct regions, namely close to the centre of UL (ORIL; Spaete & Frenkel, 1982;Weller et al, 1985) and within the inverted repeats IRs and TRs (ORIs; Stow, 1982;Mocarski & Roizman, 1982). The cis-acting signals required for ORI s activity reside within a 90 bp segment which contains an almost perfect palindromic sequence of 45 bp (Stow & McMonagle, 1983).…”

Section: Introductionmentioning

confidence: 99%

Identification of a Varicella-Zoster Virus Origin of DNA Replication and Its Activation by Herpes Simplex Virus Type 1 Gene Products

Stow

Davison²

1986

SUMMARYWe have identified and characterized an origin of DNA replication in the genome of the human herpesvirus, varicella-zoster virus (VZV). This origin of replication (VZV ORIs) is located within the major inverted repeats in a position equivalent to that occupied by one of the herpes simplex virus type 1 (HSV-1) replication origins. Products encoded by both VZV and HSV-1 activate cloned copies of VZV ORIs, generating high molecular weight molecules consisting of tandem duplications of the input plasmid. The VZV ORIs region contains a tract of alternating A and T residues located at the centre of symmetry of an almost perfect palindrome of 45 bp, and the use of plasmid deletion mutants has demonstrated that this tract is an important functional element of the origin. Two sequences common to the VZV ORIs region and the regions specifying the two HSV-1 origins (ORIs, located within the TRs/IRs regions, and ORIL, located within the UL region) were identified and these may represent important recognition sites. One is an 11 bp sequence (CGTTCGCACTT), and the other is represented by the tract of alternating A and T residues. VZV does not appear to contain an origin of replication in a position equivalent to that of HSV-10RIL.

“…This procedure has subsequently been refined by using molecularly cloned restriction fragments (Stow, 1982). Meanwhile, several groups have succeeded in defining very precisely the sequence elements of HSV replication origins Gray & Kaerner, 1984;Weller et al, 1985 ;Lockshon & Galloway, 1986) and cleavage/packaging signals (Spaete & Frenkel, 1982.…”

Section: Amplification Of Plasmids In Bhk Cells Infected With Hsvmentioning

confidence: 99%

Herpes Simplex Virus Causes Amplification of Recombinant Plasmids Containing Simian Virus 40 Sequences

Matz

1989

SUMMARYSimian virus 40 (SV40) DNA, inserted into a plasmid vector, does not replicate when transfected into baby hamster kidney cells. However, when the recipient cells are superinfected with herpes simplex virus type 1 (HSV-1), extensive amplification of the introduced plasmid occurs. Deletion of the late SV40 region or part of the coding sequences of the small tumour (t) antigen has no effect on the efficiency of amplification, whereas manipulations affecting either the SV40 origin of replication or the integrity of large tumour (T) antigen substantially decrease HSV-induced amplification. Phosphonoacetic acid, an inhibitor of HSV DNA polymerase, strongly inhibits plasmid replication. Also, an HSV-1 mutant with a temperature-sensitive defect in the DNA polymerase gene (tsH) is unable to carry out amplification of test plasmids at the non-permissive temperature. On the other hand, a further mutant (tsS) causes SV40-plasmid amplification independent of the temperature, but this mutant fails to amplify a plasmid with an HSV origin at the non-permissive temperature. Thus, HSV-induced amplification of heterologous DNA is possible in the absence of HSV DNA replication. Since tsS putatively has a defect in the gene coding for an HSV origin-binding protein (UL9), this observation appears plausible. The implications for interaction between herpesviral replication functions and heterologous (possibly cellular) DNA sequences are discussed. INTRODUCTIONInfection with herpes simplex virus (HSV) turns off the DNA replication of the host cell (Fenwick & Walker, 1978). It is, therefore, surprising that in several simian virus 40 (SV40)-transformed cell lines, SV40 DNA sequences are over-replicated upon HSV infection (Schlehofer et al., 1983(Schlehofer et al., , 1986Matz et al., 1984Matz et al., , 1985. This specific DNA amplification has been shown to depend on the herpesviral DNA polymerase (Matz et al., 1984). The structure of amplified SV40 DNA in the Syrian hamster cell line Elona has been analysed and found to consist of large concatemeric molecules (Matz, 1987). The structural similarity of the amplified DNA species with herpesviral DNA from defective interfering particles (Frenkel, 1981) supported the assumption that this illegitimate over-replication occurs under the direction of herpesviral DNA replication functions. Analysis of the amplified SV40 DNA revealed minor differences from standard SV40 DNA and failed to identify any sequence element that resembled a herpesvirus-specific origin of replication (Matz, 1987). In this report the question was addressed as to whether amplified DNA, isolated from the HSV-infected Elona cell line, or simply standard SV40 DNA can substitute for a herpesviral origin of replication in a functional assay previously designed for the identification of HSV replication origins (Stow, 1982).