1 MRC Virology Unit, Institute of Virology, Church Street, Glasgow G11 5JR, UK
2 Veterinary Medical Research Institute, Hungarian Academy of Sciences, H-1581 Budapest, Hungary
Correspondence
Andrew Davison
a.davison{at}vir.gla.ac.uk
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ABSTRACT |
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The GenBank accession numbers of the Third Party Annotations of adenovirus genome sequences reported in this paper are listed in Table 1.
Published ahead of print on 13 August 2003 as DOI 10.1099/vir.0.19497-0
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INTRODUCTION |
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Phylogeny, classification and genetic organization |
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Splicing |
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Splicing is not universal in adenoviruses: in the human viruses, E1B 19K, E1B 55K and IX are single exon genes. Nonetheless, a pattern in which a common leader is spliced to any one of several downstream protein-encoding exons is evident in the late, E2, E3 and E4 regions. This simple layout, termed here the leaderexon structure, facilitates the evolution of new genes by capture or duplication, merely requiring the presence of a splice acceptor site upstream from a newly inserted protein-encoding region. This strategy has apparently functioned throughout adenovirus evolution and is considered in further detail below. As far as can be deduced from sequence comparisons, the general splicing patterns of the late and E2 genes is common to all adenoviruses. Thus, late genes are spliced from an untranslated leader, whether tripartite, as in mastadenoviruses and atadenoviruses (Khatri & Both, 1998), or bipartite, as in aviadenoviruses (Sheppard et al., 1998
). Also, in all adenoviruses, the initiation codon for pTP is located in a short exon between pIIIa and III (Fig. 2
). This initiation codon is also utilized for expression of pol in the mastadenoviruses, but apparently not in the other genera, where the short exon is probably still spliced to the main coding exon, but pol translation is initiated in the main exon. These differences reflect minor evolutionary tinkering; in this case, the change of register in splice sites to allow the leader in the leaderexon structure to switch between being non-coding and coding. Whichever situation pertains, the structure lends itself well to evolution of new genes. Differences between the genera are also evident in splicing of DBP. This gene is probably spliced from upstream non-coding exons in all adenoviruses, but in aviadenoviruses and siadenoviruses it has accrued an additional coding exon upstream from the main exon.
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Genome sequences |
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The nucleotide composition properties of adenovirus genomes have attracted interest, with a focus on the atadenoviruses (Benk & Harrach, 1998
; Farkas et al., 2002
). Wide variation in nucleotide composition is characteristic of many groups of organisms, including adenoviruses, but the driving evolutionary forces remain elusive. Davison et al. (2000)
highlighted the fact that certain adenovirus genomes (mastadenoviruses CAdV-1 and CAdV-2, atadenovirus OAdV-7 and siadenoviruses TAdV-3 and FrAdV-1) are depleted throughout in the CG dinucleotide. In cellular genomes, this evolutionary phenomenon is thought to result from methylation of the cytosine residue in the CG dinucleotide, followed by spontaneous deamination to TG and fixation by DNA replication. CG depletion is also a feature of certain herpesviruses and has been attributed to methylation of latent genomes resident in dividing cell populations (Honess et al., 1989
). This parallel yields provocative indicators to unexplored aspects of adenovirus biology.
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Genus-common genes |
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There are 16 clearly defined genus-common genes. We presume that these were inherited from a common ancestral adenovirus, in which they were all expressed by splicing. Their primary functions are in DNA replication (pol, pTP and DBP), DNA encapsidation (52K and IVa2) and formation and structure of the virion (pIIIa, III, pVII, pX, pVI, hexon, protease, 100K, 33K, pVIII and fiber). Two additional protein-encoding regions may be added. One, 22K, originates from lack of splicing in 33K, and thus the N-terminal sequence of the protein is identical to that of 33K but the C-terminal sequence is encoded by the 33K intron. However, the putative 22K-encoding region of atadenoviruses does not extend through the intron, and thus its inclusion for this genus is tentative. The second addition is the U exon, which extends from an initiation codon to a splice donor site and is regulated by a minor late promoter (Chow et al., 1979; Davison et al., 1993
, 2000
). The downstream exons spliced to this exon have not yet been identified. They may correspond to IVa2, pol, pTP or DBP and yield differentially spliced forms of one or more of these genes encoding N-terminally extended proteins. The U exon appears to be a genus-common feature that has been lost in certain mastadenoviruses (PAdV-5 and MAdV-1).
Candidate splice sites for the majority of genus-common genes may be predicted from DNA sequences. However, particular uncertainty should be expressed about two. One gene, 33K, is poorly conserved among genera and identification of the splice sites is tentative in some cases. Also, the first exon is not visible in DAdV-1. The second problem concerns IVa2, which is involved in transcriptional activation of the late promoter and in capsid assembly and DNA packaging (Zhang & Imperiale, 2003). In mastadenoviruses, conservation of the region upstream from the first ATG codon supports splicing from an upstream protein-encoding exon. This is in accord with data that demonstrate splicing of the main coding region from a short leader close upstream, such that the five N-terminal residues of IVa2 correspond to residues within pol (Baker & Ziff, 1981
; Reddy et al., 1998a
). However, the splice sites are not conserved throughout the mastadenoviruses. In atadenoviruses, mapping data for OAdV-7 indicate that IVa2 is not spliced (Khatri & Both, 1998
), but this is at variance with conservation of the region upstream from the initiation codon, and again points to the existence of an upstream coding exon. We conclude that the transcriptional pattern of IVa2, which is likely to have been inherited by all genera, is worth further investigation.
Several adenovirus proteins (genus-common pTP, pIIIa, pVII, pX, pVI and pVIII, and genus-specific p32K of atadenoviruses) are cleaved by the protease in steps that are essential for the synthesis of infectious virus (Weber, 1995). Reported consensus cleavage sites may be summarized as (M/L/I)XGG'X and (M/L/I/N/Q)X(A/G)X'G (Anderson, 1990
; Farkas et al., 2002
; Ruzindana-Umunyana et al., 2002
; Vrati et al., 1996
; Webster et al., 1989
). Since the protease is a genus-common gene, proteolytic maturation is evidently an ancient feature of the adenovirus replicative cycle. As an example, Fig. 3
shows putative cleavage sites for all of the sequenced viruses in pX, which, along with pVII and V, generates the core proteins of the virion. The primary translation product consists of an extended, basic N-terminal region linked to a short, basic C-terminal region via a highly conserved hydrophobic domain. This protein is cleaved by the protease between the basic N-terminal and hydrophobic domains (and in some viruses at a second site nearer the N terminus) to give rise to a core protein (X or µ) that is closely associated with the virion DNA. An incidental, but provocative, observation is that unprocessed pX in all adenoviruses has the primary sequence features of a class II membrane protein.
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Genus-specific genes |
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Gene capture has played an important role throughout adenovirus evolution. Thus, genus-common genes, such as pol, IVa2 (which contains an ATP-binding domain) and protease, possibly resulted from very ancient capture events. Table 3 lists adenovirus genes with homologues in cellular or other viral genomes that have been captured more recently, after the genera diverged. Genes with cellular counterparts are taken to represent imports into adenoviruses, but those with counterparts only in other viruses could have been transferred from virus to virus in either direction. Whether discernable as captured or not, genus-specific genes range from two (E1B 55K and E4 34K) whose development pre-dated divergence of mastadenoviruses and atadenoviruses, through genes that characterize all viruses in a genus (e.g. E1A in mastadenoviruses and p32K in atadenoviruses) to genes that are specific to a subset of viruses, or even a single virus, within a genus (e.g. E3 12·5K in mastadenoviruses). This complexity in definition is not unexpected, since genes could be gained or lost at any stage.
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Evolution of E4 in the mastadenoviruses appears particularly complex. In this region, precise genetic relationships are readily catalogued between human adenovirus species, but in other mastadenoviruses the relationships are difficult to assess, although the basic structure and expression pattern appear to be conserved. As a result, genetic relationships between non-primate mastadenovirus E4 genes are not specified in Table 2. In five of the human adenovirus species, E4 contains six leftward-oriented genes (ORF1, ORF2, ORF3, ORF4, 34K and ORF6/7), transcripts from which are regulated by a promoter near the right end of the genome. ORF6/7 mRNA results from further splicing between the 5' end of 34K and the region immediately downstream of 34K, and thus the ORF6/7 and 34K proteins share N-terminal sequences. HAdV-F is unusual in lacking a counterpart to ORF1, presumably as a result of deletion. ORF1 appears to be derived from a captured dUTPase gene, but its descendents in human adenoviruses have not retained the active site residues and presumably carry out other functions (Weiss et al., 1997
). Evolution of E4 in mastadenoviruses has evidently involved duplication or deletion events resulting in variable numbers of genes. Occasionally, alternative routes of functional partition for duplicated 34K or dUTPase-derived genes have led to a situation where sequence similarity between two viruses is greatest between ORFs that do not correspond in location. In atadenoviruses, knowledge of E4 is less extensive, but splicing in leaderexon fashion and gene duplication are evident. Two tandem 34K genes (34K-1 and 34K-2) are present, and the RH family of duplicated genes (termed ORF8 and ORF9 in DAdV-1) encoding F-box proteins has developed upstream (Both, 2002b
). Two related genes (ORF5 and ORF6) resulting from duplication are present at the right end of the DAdV-1 genome.
These observations lead to a speculative model for the evolution of E4 in mastadenoviruses and atadenoviruses in which 34K was present in the common ancestor and other genus-specific genes were inserted nearer to the right genome terminus. These included a dUTPase gene in the mastadenovirus lineage and an F-box gene in the atadenovirus lineage. The 34K, dUTPase and F-box genes then proliferated at various stages by duplication, divergence and functional partition, and sometimes by deletion, to give rise, in concert with development of unrelated additional genes, to the E4 formats observed. The dUTPase-derived proteins in modern mastadenoviruses exhibit a range of degrees of relatedness. Most are probably not active dUTPases, but a functional enzyme appears to have been retained in the lineages leading to TSAdV-1 and PAdV-5/BAdV-2. Other clues of gene duplication in E4 also remain, such as in two 34K-derived genes in PAdV-5 and in three genes in TSAdV-1 that are related to ORF2 of primate mastadenoviruses. However, we suspect that divergence of duplicated genes may have proceeded so far in many instances as to obliterate evidence of common origin. It is also interesting to note that duplication of a dUTPase gene has occurred during herpesvirus evolution (McGeoch, 1990), where it is postulated that the initial duplication event resulted in a fused, double-length gene encoding two sets of active site residues. This was followed by loss of one active site to yield a still-active enzyme, and in one lineage by loss of the remaining active site to end in a protein that is presumably no longer a dUTPase (McGeoch & Davison, 1999
).
In aviadenoviruses, E4 is substantially larger than in other genera. Understanding of the gene content is incomplete, but useful information on transcription of the FAdV-1 and FAdV-9 genomes (Ojkic et al., 2002; Payet et al., 1998
) has aided our extension of previous analyses. It is clear that splicing is common and that gene capture, duplication and functional partition have occurred. A family of putative glycoprotein genes is located near the right genome end in FAdV-1 and FAdV-9. It consists of three rightward-oriented genes (ORF9, ORF10 and ORF11) in the former and one rightward- (ORF11) and one leftward-oriented gene (ORF23) in the latter. The origin of this gene family is revealed by the clear similarity between the ORF11 protein from each virus and cellular leukocyte adhesion molecules. In the absence of obvious cellular forerunners, two observations currently imply that genetic exchange may also have occurred between avian adenoviruses and herpesviruses. Firstly, the ORF19 proteins in FAdV-1 and FAdV-9 are most closely related to membrane proteins (putative lipases) encoded by members of the genus Mardivirus, an avian lineage of the Herpesviridae (subfamily Alphaherpesvirinae) that includes Marek's disease virus (Ojkic & Nagy, 2000
). Secondly, partial sequence data indicate that the gene (ORF4) at the right end of the FAdV-10 genome (AF160185) lacks counterparts in FAdV-1 and FAdV-9, but has relatives in several other viruses (Davison et al., 2003
). ORF4 is predicted to be spliced, and has closest relatives again in mardiviruses. Distant relatives of this gene are detectable in two other lineages of the Herpesviridae (subfamily Betaherpesvirinae and an amphibian herpesvirus) and in one lineage of the Poxviridae (fowlpox virus).
Gene capture and duplication also feature in E1. An atadenovirus protein (p32K) bears a tenuous relationship to small acid-soluble proteins of bacteria (Él et al., 2003
), and the siadenoviruses are so named because they encode a putative sialidase (Davison & Harrach, 2002
). The aviadenoviruses have a dUTPase (ORF1), which retains active site residues, plus a parvovirus Rep protein (ORF2) (Chiocca et al., 1996
). Although Chiocca et al. (1996)
speculated that the dUTPase genes of mastadenoviruses and aviadenoviruses may have evolved via transfer of an ancestral gene from one genome terminus to the other, it is equally likely that they were acquired by separate capture events. Duplicates of aviadenovirus ORF2 appear to be present on the opposing strand (ORF12 and ORF13), and are expressed by splicing from the short coding exon utilized by pTP.
In contrast to E1 and E4, which are present in all genera, E3 features only in mastadenoviruses and siadenoviruses. This location for genus-specific genes may have been arrived at independently, or may represent an ancient locus for rapid gene evolution that has been lost in two genera. A substantial set of genes, numbering up to nine, has evolved in mastadenovirus E3. The two genes at the ends of this block (12·5K and 14·7K) encode distantly related proteins that probably arose via gene duplication at an early stage in mastadenovirus evolution with subsequent loss in some lineages. The intervening genes encode membrane proteins, certain of which (CR1 genes) in primate adenoviruses have relatives in primate cytomegaloviruses (a lineage of subfamily Betaherpesvirinae in the Herpesviridae). CR1 genes share a common motif but are highly variable in number and sequence in both virus families (Davison et al., 2003). Interestingly, TSAdV-1 lacks CR1 genes in E3, but the cognate domain is present in the putative glycoprotein encoded by a gene (105R-T), which is unique to this virus and situated at the right end of the genome. Both (2002b)
detected a weak similarity between the single siadenovirus E3 protein and RH5 of atadenoviruses OAdV-7 and BAdV-4, but the evolutionary significance of this is not clear.
In the genomes of most primate mastadenovirus species (including all human and chimpanzee viruses), the region between the pTP and 52K genes contains one or two rightward-oriented VA RNA genes, which are transcribed by RNA polymerase III (pol III) (Kidd et al., 1995; Ma & Mathews, 1996
; Mathews & Shenk, 1991
). The encoded partially double-stranded RNAs are approximately 160 nucleotides in size, and are involved in translational control and inhibition of the interferon response (Mathews & Shenk, 1991
; Mori et al., 1996
). A 90 nucleotide pol III RNA is also produced by a leftward-oriented gene located between ORF16 and ORF9 in FAdV-1 (Larsson et al., 1986
). Thus, acquisition of VA RNA genes is likely to have occurred at least twice during adenovirus evolution, once in primate mastadenoviruses (perhaps from a tRNA gene, followed by gene duplication in some lineages) and once in aviadenoviruses. On the basis of limited sequence similarity to FAdV-1, a candidate VA RNA gene was identified in the DAdV-1 genome, overlapping the 3' end of ORF4 (Hess et al., 1997
). This region is absent from the other two atadenoviruses sequenced, and functional investigations have failed to detect a VA RNA in OAdV-7 (Venktesh et al., 1998
). If the identified DAdV-1 VA RNA gene is genuine, its evolution might have been independent or might have involved transfer to or from an aviadenovirus.
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Evolution |
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The most recent ancestor of all modern adenoviruses is likely have been an adenovirus that existed before the divergence of bony fish from other vertebrates. This virus possessed a substantial prior evolutionary history. Since adenoviruses of invertebrates have not yet been discovered, the characteristics of adenoviruses predating vertebrates are unknown. Nonetheless, tantalizing glimpses may be had into earlier epochs. There are clear similarities in overall architecture of the virion and in the structure of its principal protein component (hexon) between adenoviruses and bacteriophage PRD1 (Belnap & Steven, 2000; Benson et al., 1999
, 2002
; San Martin & Burnett, 2003
). PRD1 belongs to the family Tectiviridae, infects Gram-negative hosts and has a linear, double-stranded DNA genome of 15 kbp that is linked to a TP (Bamford, 2002
; Bamford & Ackermann, 2000
). Adenovirus hexon possesses the jellyroll fold common to capsid proteins of many viruses (Chelvanayagam et al., 1992
), but the structural relationship is closest to that of PRD1. Parallels also extend to other features, such as fiber and its PRD1 counterpart (spike), which are present at the virion vertices. These findings provide evidence for divergent evolution of adenoviruses and tectiviruses from an ancestor that pre-dated eukaryotes and exhibited the adenovirus morphology. The ancient origins of this morphology are highlighted further by recent findings on bacteriophage Bam35, which infects a Gram-positive host. PRD1 and Bam35 are morphologically indistinguishable and share the hexon fold, even though they are thought to have diverged over a billion years ago (Ravantti et al., 2003
).
Protein-primed DNA replication is employed by adenoviruses and certain bacteriophages (Berencsi et al., 1995; de Jong et al., 2003
; Liu et al., 2003
; Salas, 1991
). The components are a linear double-stranded DNA template with ITRs, pol, TP and at least one DBP. This strategy is used by PRD1 (Bamford et al., 1991
) and by bacteriophage
29 (19 kbp), which belongs to the Podoviridae and has a different capsid morphology from PRD1 (Pe
enková & Pa
es, 1999
). Moreover, in adenoviruses and these two bacteriophages, TP and pol are early genes arranged in tandem near the left genome end, and the late genes are located more centrally, adjacent to TP and pol and arrayed rightward. The antiquity of protein-primed DNA replication is further underscored by its occurrence in linear plasmids of fungi and plants, which generally encode the required pol and TP (Paillard et al., 1985
; Rohe et al., 1991
), and by linear bacterial genomes of Streptomyces species (Chen, 1996
).
In summary, we may speculate that the protein-primed DNA replication strategy originated at a very early stage in evolution, to be followed by acquisition of the adenovirus morphology during a pre-eukaryotic era. Introduction of splicing and additional replicative and structural genes resulted in an adenovirus from which extant members of the family have inherited at least 16 genes. Subsequent lineages developed specific subsets of genes that fit them to particular biological niches.
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ACKNOWLEDGEMENTS |
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