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Adenoviruses and human misery
History
(1953) first report of adenoviruses cultured from tonsils
and adenoids; (1962) Adenovirus type 12 shown to cause tumors in
rodents (hamsters); (1977) first demonstration of mRNA splicing in
adenoviruses; (1988) adenovirus proteins shown to interact with
cellular tumor suppressor proteins. Despite evidence for adenovirus
oncogenicity in rodents and in tissue culture they have never been
strongly associated with any human cancer.
Diseases
There are 42 adenovirus serotypes with five new types
awaiting classification. Adenoviruses can infect the respiratory
tract; eye, gastrointestinal tract and bladder. (CNS infection has
been documented but is very rare). Most adenovirus disease is
caused by only a subset of the 42 types (one third) and most
infections are subclinical.
-- 5% of acute respiratory disease in children under 5 years of age
is caused by adenoviruses and 10% of the pneumonias. Ad.
infections are difficult to distinguish from influenza,
parainfluenza and RSV. Conjunctivitis can occur with respiratory
illness in such cases the disease is called pharyngoconjunctival
fever.
-- Acute respiratory disease (ARD) is commonly seen in military
recruits probably due to fatigue and crowding in barracks. Ad.
types 4 and 7 are responsible for these outbreaks and a vaccine is
available.
-- Eye infections characterized by a mild conjunctivitis "swimming
pool conjunctivitis" are caused by adenoviruses and have been
linked to transmission in contaminated swimming pools.
--Ad. types 8 and 37 can cause a more severe illness known as
epidemic keratoconjunctivitis (EKC). Corneal opacity with
concomitant vision loss in 10% of cases.
--Latency ??? I hope so.
--Epidemiology: adenoviruses are highly species specific (it's safe
to pet your dog). Fecal oral transmission is common in children.
STRUCTURE AND BASIC PROPERTIES
Adenoviruses are nonenveloped with an icoshedral structure and a
dsDNA genome of 36 kb. The architecture of the virion is unique
resembling a WWII mine or a space satellite. Projecting from each
of the twelve vertices is the fiber. The protein coat (capsid) is
comprised of 252 capsomeres (240 hexons and 12 pentons). penton =
penton base + the fiber. Inside the capsid is the viral genome
which has the terminal polypeptide (TP) covalently linked to the 5'
end at a dCMP residue. Adenoviruses have inverted terminal
redundances comprised of repeats of 100-140bp that vary in number
with each serotype. Within the core, polypeptides V and VII are
noncovalently linked to the viral DNA. Interestingly, soluble
pentons have been shown to be toxic to cells. Adenoviruses are
classified within the family Adenoviridae with two genera
Mastadenovirus and Aviadenovirus. Human adenoviruses have been
classified into six subgroups based on their hemagglutination
properties, tumorigenicity, transformation of cells in culture and
G+C percentage.
REPLICATIVE CYCLE
The adenovirus replicative cycle is divided into early and late
phases with the late phase occurring when viral DNA replication
begins. Normally structural proteins are the major polypeptides
synthesized during the late phase. This division into early and
late is over-simplified and somewhat misleading as we will see in
upcoming revelations. After infection adenoviruses rapidly
shutdown host cell macromolecular synthesis i.e. cell DNA and
protein synthesis. The mechanism of shutoff is not clear but
protein synthesis is rapidly inhibited whereas cell DNA synthesis
is shut down at a more leisurely pace. The adenovirus lytic cycle
is very efficient producing 10,000 virions per cell with one virus
cycle occurring in 32-36 hours.
ATTACHMENT-PENETRATION-UNCOATING
Adenovirus attachment is mediated by the fiber which binds a
specific receptor on the cell membrane. Subsequently the attached
virus migrates to clathrin coated pits to form a receptosome and
become internalized. A pH drop in the receptosome alters virion
surface properties and results in virion release (with the loss of
some viral capsid protein) into the cytoplasm of the cell. The
capsid (or what is left of it) migrates to the nucleus via
microtubules and viral DNA enters the nucleus (home at last)
through nuclear pores. Many if not most virion proteins remain in
the cytoplasm (sorry guys). This whole process requires about 2
hours (at 37oC) and will not occur at 0øC. Finally viral DNA is
converted into a cell histone complex and may attach to the nuclear
matrix for replication.
EARLY TRANSCRIPTION
Viral gene expression is not a haphazard process. On the contrary
it is highly ordered and carefully orchestrated in much the same
manner as genes are regulated for cell division or embryonic
development. The ability to function efficiently is critical to the
virus's success in a hostile environment where it is dependent on
the host cell for basic macromolecular machinery and supplies. RNA
polymerase II is responsible for viral gene transcription at both
early and late times. Early RNA synthesis occurs from at least 7
distinct regions of the viral genome, from separate promoters and
from both DNA strands. Extensive splicing occurs for both early and
late transcripts, an observation that was first documented in
adenoviruses. Recent evidence has led to further qualification and
subdivision of early transcription. Studies with the protein
synthesis inhibitors cycloheximide and anisomycin have shown a
defined order of mRNA expression.
immediate early -- L1
pre-early -- E1A
delayed early -- E1B, E2A, E2B, E3, E4
intermediate -- IVa2, IX
Rightward transcription.
E1A - transformation, viral gene transcription
E1B - transformation
E3 - nonessential in tissue culture, immune modulation in vivo?
L1 - function unknown
Leftward transcription.
E4- immune modulation
E2A - DNA binding protein (DBP)
E2B - DNA polymerase (140kd) and 80 kd precursor to terminal
protein (pTP)
Regulation of early gene expression. The E1A region is pivotal in
early gene synthesis. The major product of the E1A is a 13S mRNA
which encodes a 289 amino acid protein with diverse functions
including the induction of DNA synthesis, induction of mitosis
(transformation) and transactivation of viral genes. E1A controls
E1B, E2, E3, and E4 mRNA accumulation but cannot itself bind DNA.
E1A products appear to activate a series of host proteins which
bind to target sequences within early gene promoters.
Early proteins
Tumor antigens produced in hamsters bearing
adenovirus induced tumors were the first source of information on
early proteins. Antisera from these animals reacted with
adenovirus infected cells. Since early regions E1A and E1B are the
only areas commonly present in tumor cells this led to the early
characterization of proteins from these two regions. Subsequent
studies employing mRNA hybrid selection and in vitro selection
provided more definitive locations for many of the early proteins.
Region E1
This region is essential for adenovirus transformation
and both E1A and E1B are required for full transformation. In
transformation assays on primary cells in which two oncogenes are
required it has been demonstrated that E1A can cooperate with ras
and that E1B can cooperate with myc to achieve full oncogenic
transformation. Recently it has been demonstrated that E1A protein
can bind the tumor suppressor gene Rb105 (Retinoblastoma 105 kd)
and that E1B protein can bind the p53 tumor suppressor protein. In
highly tumorigenic strains of adenovirus the E1A region down
regulates MHC expression.
The E1A region produces at least six different polypeptides
ranging in size from 38 to 51 kd. The variability in molecular
weight is due in part to post-translational modification of the
proteins. Two major RNA products are produced by the E1A: 13S and
12S. The 13S mRNA encodes a 289 amino acid protein (51kd) which
binds the Rb gene product. The 12S mRNA encodes a 243 amino acid
protein (48kd). These two proteins differ only by 46 amino acids
which are spliced from the 12S mRNA.
The E1B region encodes 3 polypeptides of 19kd, 20kd and 53-
58kd. The 19kd and 53-58kd proteins are important in cell
transformation. The 19kd protein transactivates E1A, E1B, E2, E3,
E4 and cellular genes such as the heat shock gene. The 55kd (53-
58kd) protein binds the p53 tumor suppressor protein which is also
bound by the SV-40 large tumor antigen. Furthermore the 55kd
protein interacts with the E4 34kd protein to support efficient
synthesis of viral DNA, expression of late genes and host cell shut
off.
Region E2
This region is subdivided into two separate
transcription regions: E2A and E2B. The E2A region encodes for a
single stranded DNA binding protein (DBP) which is heavily
phosphorylated at the N terminus. DBP is required for DNA
replication and probably also functions in the regulation of
transcription. The E2B region encodes for the precursor to the
terminal protein (80kd) that is cleaved during viral assembly to
55kd while covalently bound to DNA. This region also encodes the
140kd DNA polymerase.
Region E3
This region is nonessential in tissue culture and can
be deleted or replaced without disrupting viral replication. It
encodes a 19kd protein that blocks MHC transport to the plasma
membrane and a 14.7kd protein that inhibits lysis of adenovirus
infected cells by tumor necrosis factor (TNF). In addition, it
encodes a 10.4kd protein which binds to the EGF receptor. Thus,
the E3 region seems to contain genes which are involved in the
modulation of host response to infection.
Region E4
This region encodes a number of polypeptides and at
least two of its products have been assigned a function. The 11kd
protein binds the nuclear matrix and a 34kd protein binds to the
E1B 55kd protein.
DNA REPLICATION
Adenovirus DNA replication has been studied both in vitro and
in vivo. In fact, adenovirus was the first DNA virus to be
successfully replicated in an in vitro system. At least three
viral products and four host cell products have been identified
which are essential for viral DNA synthesis. Adenovirus
replication occurs in the nucleus and is semiconservative with each
strand being elongated continuously without Okazaki intermediates.
The viral origin of replication is located in the termini of the
viral genome. Two types of replication are thought to occur. In
type I, strand elongation occurs from duplex DNA with strand
displacement. In type II replication occurs from a single stranded
template possibly a panhandle type molecule. Because the template
is linear not circular priming of synthesis occurs by covalent
attachment of a nucleotide to the terminal protein (protein priming
model).
Viral proteins required for replication: DNA binding protein
(DBP); precursor terminal protein (80kd, pTP) and 140 kd viral DNA
polymerase.
Cellular proteins required for adenovirus DNA replication:
1. nuclear factor I (NFI); binds the adenovirus origin of
replication and is involved initiation and elongation.
2. nuclear factor II (NFII) is a type 1 topoisomerase
3. nuclear factor III is a DNA binding protein that recognizes the
sequence ATGCAAAT.
4. ORP A, binds within the first twelve nucleotides of the viral
genome.
LATE TRANSCRIPTION
Control of late transcription is very complex and little is
known about the molecular mechanisms involved in regulating the
switch from early to late gene expression. One of the major
features of late transcription is the presence of a tripartite
leader for late mRNA. Synthesis of late transcripts begin at 16.45
map units and extend to 99 map units. Extensive splicing of this
large transcript then occurs. In general their are 5 classes of
late transcripts which have variable 5'ends and coterminal 3' ends.
VA RNAs. Virus associated RNAs known as VA RNA I and VA RNA II are
small (155 bases) RNAs generated by pol III. They do not encode
polypeptides and have the potential to form extensive secondary
structure. Suggested functions for these RNAs particularly VA I
include: 1. regulation of late mRNA splicing; 2. control of the
rate of translation of late polypeptides and 3. inhibition of the
effects of interferon by blocking binding of dsRNA to cellular
protein kinase and by binding the kinase and blocking eIF2
inactivation.
Late proteins
The synthesis of late proteins is maximal 20 hr
post-infection. Most late proteins are structural components of
the virion but some early genes are also made late.
Techniques of note:
Hybrid selection\ in vitro translation
Hybrid arrested translation (HART)
heteroduplex analysis
S1 nuclease mapping
in vitro replication
UV mapping of transcripts
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