Capsid Structure of Simian Cytomegalovirus from Cryoelectron Microscopy: Evidence for Tegument Attachment Sites

This Article

	Abstract
	Full Text (PDF)
	An erratum has been published
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Trus, B. L.
	Articles by Steven, A. C.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Trus, B. L.
	Articles by Steven, A. C.

Previous Article | Next Article

Journal of Virology, March 1999, p. 2181-2192, Vol. 73, No. 3
0022-538X/99/$00.00+0

Capsid Structure of Simian Cytomegalovirus from Cryoelectron Microscopy: Evidence for Tegument Attachment Sites

Benes L. Trus,¹^,² Wade Gibson,³ Naiqian Cheng,¹ and Alasdair C. Steven¹^,^*

Laboratory of Structural Biology, NIAMS,¹ and Computational Bioscience and Engineering Laboratory, CIT,² National Institutes of Health, Bethesda, Maryland 20892, and Virology Laboratories, Johns Hopkins School of Medicine, Baltimore, Maryland 21205³

Received 9 September 1998/Accepted 16 November 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

We have used cryoelectron microscopy and image reconstruction to study B-capsids recovered from both the nuclear and the cytoplasmicfractions of cells infected with simian cytomegalovirus (SCMV).SCMV, a representative betaherpesvirus, could thus be comparedwith the previously described B-capsids of the alphaherpesviruses,herpes simplex virus type 1 (HSV-1) and equine herpesvirus 1 (EHV-1),and of channel catfish virus, an evolutionarily remote herpesvirus.Nuclear B-capsid architecture is generally conserved with SCMV,but it is 4% larger in inner radius than HSV-1, implying thatits ~30% larger genome should be packed more tightly. IsolatedSCMV B-capsids retain a relatively well preserved inner shell(or "small core") of scaffolding-assembly protein, whose radial-densityprofile indicates that this protein is ~16-nm long and consistsof two domains connected by a low-density linker. As with HSV-1,the hexons but not the pentons of the major capsid protein (151kDa) bind the smallest capsid protein (~8 kDa). Sodium dodecylsulfate-polyacrylamide gel electrophoresis showed cytoplasmicB-capsid preparations to contain proteins similar in molecularweight to the basic phosphoprotein (~119 kDa) and the matrix proteins(65 to 70 kDa). Micrographs revealed that these particles hadvariable amounts of surface-adherent material not present on nuclearB-capsids that we take to be tegument proteins. Cytoplasmic B-capsidswere classified accordingly as lightly, moderately, or heavilytegumented. By comparing the three corresponding density mapswith each other and with the nuclear B-capsid, two interactionswere identified between putative tegument proteins and the capsidsurface. One is between the major capsid protein and a proteinestimated by electron microscopy to be 50 to 60 kDa; the otherinvolves an elongated molecule estimated to be 100 to 120 kDathat is anchored on the triplexes, most likely on its dimer subunits.Candidates for the proteins bound at these sites are discussed.This first visualization of such linkages makes a step towardsunderstanding the organization and functional rationale of theherpesvirustegument.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Herpesvirus form an extensive family of DNA viruses, whose host range encompasses much of the animal kingdom. They are classifiedinto three subfamilies alpha-, beta-, and gammaherpesviruses,on the basis of biological properties [53]. Despite this diversity,their assembly pathway is closely conserved: the nucleocapsidis formed in the nucleus and follows a pathway that bears a markedresemblance to those of DNA bacteriophages (8, 14). First,a procapsid is assembled, which then releases its morphogenicinternal scaffolding protein and becomes filled with DNA, concomitantwith a major conformational transition of the capsid shell. Subsequentevents, however, are not phage-like. The nucleocapsid exits thenucleus and acquires its tegument (53) and lipoprotein envelope.The latter events remain a focus of active research and some controversy(see, for example, references 13, 26, 51, and 63).

Although virion assembly is a continuous sequential process, several kinds of capsids have been identified as representingstable endpoints or long-lived states. They include A-capsids,empty shells thought to arise from abortive attempts to packageDNA or its aberrant release; C-capsids, which are filled withDNA; and B-capsids, which contain internal proteins but littleor no DNA (for reviews, see references 28, 49 and 62). "B-capsid"refers either to an intranuclear capsid visualized in situ thatcontains internal material with different staining propertiesfrom the DNA in C-capsids (which we interpret as mainly scaffolding-assemblyprotein) or to a capsid isolated from the nuclear fraction thatcontains scaffolding proteins but little or no DNA. Here, we relaxthe requirement for nuclear provenance and refer to nuclear andcytoplasmic B-capsids, respectively. It now appears that thereare several kinds of B-capsids. "Large-cored" B-capsids correspondto the normally short-lived and infrequently observed procapsid(42, 47). "Small-cored" B-capsids (49) derive from large-coredB-capsids and have a mature surface shell. It remains unclearwhether these particles represent an assembly intermediate oran abortive byproduct (56) or how many subclasses they maycomprise.

As noted above, herpesvirus capsid assembly is a conservative process. The current paradigm is that the surface shell is aT=16 icosahedron containing three essential proteins. Nine hundredsixty copies of the major capsid protein (M_r $sime$ 120,000 to 155,000,depending on the virus) make up 150 hexons and 12 pentons. Theother two proteins form the triplexes, complexes that are presenton the outer surface at the 320 sites of local threefold symmetryand have an $alpha$ ₂ $beta$ stoichiometry (43). Typically, the $alpha$ -proteinhas a mass of 33 to 35 kDa, and the mass of the $beta$ -protein is eithersimilar or in the 50-kDa range (10). Most herpesvirus capsidsalso contain an additional low-molecular-weight protein that bindsaround the rims of hexons but not to pentons (11, 65, 72,73).

The above account owes most to observations relating to herpes simplex virus type 1 (HSV-1), the archetypal alphaherpesvirus.However, one property of herpesviruses that does not suggest animmutable capsid structure is their variation in genome size,which ranges from ~120 to ~230 kbp (18). Betaherpesviruses accountfor three of the eight herpesviruses known to cause disease inhumans and include the cytomegaloviruses (CMVs), which have thelargest of all known herpesvirus genomes (4). Although theoverall structure of the herpesvirus capsid appears to be conserved,it has not been clear whether there are features specific to eachsubfamily. To investigate this possibility, we have used cryoelectronmicroscopy to study isolated capsids of simian CMV (SCMV), a closeand experimentally more tractable relative of human CMV (HCMV)[24].

A second motivation for this study was that it might offer insight into tegumentation. Nonenveloped capsids have been observedin significant numbers in the cytoplasms of cells infected withCMV (57) and appear to be at least partly tegumented (24,30). We have noticed that, late in the infection of culturedcells with SCMV, B-capsids appear in the cytoplasmic fraction,and these cytoplasmic B-capsids differ from nuclear B-capsidsin several respects, including their state of tegumentation. Here,we characterize the structures of nuclear and cytoplasmic B-capsidsat a resolution of ~2.2 nm and, by quantitative comparison betweenthem, identify sites of tegumentattachment.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Virus, cells, and capsid preparation. The Colburn strain of SCMV was grown in human foreskin fibroblasts prepared and infected as described earlier (24). Muchof the capsid recovery procedure has also been described (33).In brief, 5 days after infection when the cytopathic effect wasextensive and many cells were beginning to detach and float, allcells (~5 × 10⁷) were scraped into the medium, collected by centrifugation (1,500× g, 5 min, 4°C), and suspended in PB buffer (150 mM NaCl, 40mM phosphate; pH 7.4) containing 0.5% Nonidet P-40 (NP-40; BDHLaboratory Supplies, Poole, United Kingdom), at 1.0 × 10⁸ cells per ml. After 5 min on ice, the detergent-treated cellswere subjected to centrifugation (1,500 × g, 5 min, 4°C), yieldinga supernatant (NP-40 cytoplasmic fraction) and pellet (NP-40 nuclearfraction). The NP-40 nuclei were suspended in 1.5 ml of PB andlysed by 10 passages back-and-forth through a hypodermic syringewith a 23-gauge needle. After clearing the lysate of particulatematerial by centrifugation (16,000 × g, 2 min, 4°C), the resultingsupernatant and the NP-40 cytoplasmic fraction were subjectedto rate-velocity sedimentation in sucrose gradients (15 to 50%sucrose [wt/wt] in PB buffer; 40,000 rpm, 20 min, 4°C; BeckmanSW41 rotor). After centrifugation, light scattering bands wereobserved in both gradients at the position corresponding to B-capsids(24). These bands were collected by aspiration through the wallof the centrifuge tube, diluted 1:1 with PB buffer, and concentratedby pelleting (35,000 rpm, 2 h, 4°C; SW41rotor).

Protein analysis. Capsid proteins were separated by sodium dodecyl sulfate-polyacrylamide electrophoresis (SDS-PAGE), essentially as describedpreviously (39) but with a Tris-Tricine buffer system (54)and a 10 to 20% gradient gel (Novex, San Diego, Calif.). Samplesof the same nuclear and cytoplasmic B-capsid preparations usedfor cryo-electron microscopy and image reconstruction were subjectedto SDS-PAGE (150 V for 60 min). Proteins were stained with Coomassiebrilliant blue; the gel was then destained, dried, and digitizedby optical scanning. Stained proteins were quantified by usingthe Quant mode of MacBas 2.5 software (Fuji Film Co., Tokyo, Japan)after the linear range was established with an optical densitywedge.

Cryoelectron microscopy. Immediately prior to specimen preparation, capsid suspensions at a 1- to 2-mg/ml protein concentration were vortexed for 30s on a G-560 Vortex (Daigger Scientific Industries, Inc.) to disperseaggregates. Thin film specimens were formed over holey carbonfilms and vitrified by quenching them in liquid ethane cooledby liquid nitrogen according to standard procedures (9, 16).Specimens were observed in a Philips CM120 electron microscopeequipped with a liquid N₂-cooled model 626 Cryoholder (Gatan,Pleasanton, Calif.) and anticontamination blades. The grids weresurveyed at low magnification for areas with ice of suitable thicknessand appropriate particle concentrations by using a Gatan RMC 794slow-scan charge-coupled device camera. Micrographs were recordedon Kodak SO-163 film at a nominal magnification of ×36,000 byusing low-dose procedures. For size calibration, SCMV capsidswere mixed with purified T4 bacteriophages, and the axial spacingof the T4 tail sheath was used to calibrate the dimensions ofcapsids recorded in the same micrographs (10).

Image processing and reconstruction. Images used in this analysis were evaluated by optical diffraction, and the best images were scanned at 0.70 nm/pixel witha Perkin-Elmer 1010MG microdensitometer. The software and procedureswere as described earlier (2, 22, 23). These images hadtheir first zeros of the contrast transfer function (CTF) at frequenciesvarying from (1.9 nm)¹ to (2.5 nm)¹. For those images whose first zero frequency was less than (2.2nm)¹, we computationally inverted the phases of the Fourier termsbeyond the zero, i.e., in the second lobe of the CTF. Particleswere extracted from the scanned fields and preprocessed by a semiautomaticprocedure (17). For the nuclear B-capsid reconstruction, initialestimates of the orientation angles were obtained for a base setof particles by the polar Fourier transform (PFT) method of Bakerand Cheng (1), with an appropriately scaled map of HSV-1 B-capsids(17) taken as starting model. Using these orientations, a densitymap was calculated and used in the first of several subsequentcycles of PFT-based refinement of these particles' orientationsand to solve additional particles. The final reconstruction combined350 capsids from five micrographs into a three-dimensional densitymap with a resolution of 2.2 nm, according to the FRC3D criterion(17).

Cytoplasmic B-capsids were divided by visual criteria into three classes: lightly, moderately, and heavily tegumented. Thethree classes were analyzed separately, and corresponding mapswere calculated, by using the nuclear B-capsid as a starting modelin each case. The lightly tegumented capsid map included 121 capsidsfrom 4 micrographs for a resolution of 2.2 nm; the moderatelytegumented map included 257 capsids from 16 micrographs for aresolution of 2.2 nm; and for the heavily tegumented capsids,79 images from the same 16 micrographs were used for a resolutionof 2.5 nm. The smaller number of the latter particles reflectsboth their relative rarity and a lower success rate in determiningreliable orientations. To calculate the radial density profileof the inner shell, 15 particles with seemingly well preserved,i.e., round and symmetrical, cores were selected, their surfaceshells were stripped away (3), and their exposed cores werealigned by cross-correlation methods and then averaged. Furthernoise reduction was effected by azimuthal averaging, and fromthis projection a radial density profile was calculated (61).

To estimate the molecular weights of the two tegument proteins, their volumes were estimated and expressed as masses by usinga conversion factor of 0.78 kDa/nm³. To obtain the volume estimates, portions of the difference maps(moderately tegumented minus nuclear) and (heavily tegumentedminus moderately tegumented) were excised in which the respectivemolecules were well represented (see Fig. 5c and d). The numbersof voxels in the corresponding envelopes of continuously connecteddensity were then calculated. For the capsomer-capping protein,the molecule overlying the penton was used. Two estimates of volumewere obtained in each case and define the limits of the rangequoted (see Results). They represent the use of differing contourlevels and correspond respectively to the nuclear capsid containing100 or 120% of the expected mass (17).

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Nuclear and cytoplasmic B-capsids: protein composition. Cultured human fibroblasts were harvested 5 days after infection and separated into nuclear and cytoplasmic fractions aftertreatment with the detergent NP-40 to disrupt membranes. B-capsidswere then isolated from both fractions by rate-velocity sedimentationthrough sucrose gradients. Their protein compositions were thenevaluated by SDS-PAGE (Fig. 1) and are indistinguishable withrespect to their contents of capsid proteins (i.e., MCP, AP, mCP,mC-BP, and SCP in Fig. 1). They differed, however, in that cytoplasmicB-capsids contain several proteins whose electrophoretic mobilitiescorrespond to those of proteins previously classified as tegumentcomponents (24, 25, 28, 67), the strongest of which isthe 119-kDa basic phosphoprotein (BPP; also called pp150 for HCMV).There are also several closely spaced bands in the size rangeof the 69-kDa upper-matrix protein (UM; also called pp71 for HCMV)and the 66-kDa lower-matrix protein (LM, also called pp65 forHCMV), as well as a small amount of the 205-kDa high-molecular-weightprotein. None of these SCMV tegument proteins has been clonedand sequenced, but each appears to be the counterpart of an HCMVprotein that has been so characterized (25).

View larger version (22K):
[in this window]
[in a new window]

FIG. 1. Comparison of the protein compositions of nuclear and cytoplasmic B-capsids of SCMV (Colburn) by SDS-PAGE with protein detection by staining with Coomassie brilliant blue. Additional proteins are present in the cytoplasmic capsid preparation. Abbreviations (25, 28): HMWP, high-molecular-weight protein (205 kDa, homolog of HCMV UL48 protein); MCP, major capsid protein (151 kDa, homolog of HCMV UL86 protein); BPP, basic phosphoprotein (119 kDa, homolog of HCMV UL32 protein); "mp" refers to the several bands in the molecular-weight range of the upper- and lower matrix proteins (UM, 69 kDa, is the homolog of HCMV UL82 protein, and LM, 66 kDa, is the homolog of HCMV UL83 protein); AP, assembly protein (30 kDa, mature form, i.e., proteolytically processed; homolog of HCMV UL80.5 protein); mCP, minor capsid protein (35 kDa, homolog of HCMV UL85 protein); mC-BP, minor capsid binding protein (33 kDa, homolog of HCMV UL46 protein); SCP, smallest capsid protein (~8 kDa, homolog of HCMV UL48/49 protein).

Nuclear and cytoplasmic B-capsids: morphology. Typical cryomicrographs of both capsid preparations are presented in Fig. 2. Nuclear B-capsids (Fig. 2a) have a thick-walledouter shell with peripheral serrations. The angularity of a givenprojection and the sharpness of its serrations vary accordingto the viewing direction, as with equine herpesvirus 1 (EHV-1)(3) and HSV-1 (e.g., references 43 and 73). The only markeddifference between nuclear B-capsids of SCMV and those of thealphaherpesviruses is their inner ring of density, which representsthe projection of an internal protein shell. This ring is presentin >90% of these capsids, the remainder being empty, like A-capsids.As discussed below, we interpret this internal structure to bethe "small core" previously described in in situ electron microscopicobservations of B-capsids (e.g., reference 47).

View larger version (143K):
[in this window]
[in a new window]

FIG. 2. Cryoelectron micrographs of purified SCMV B-capsids (nuclear [a] and cytoplasmic [b]). (b) Several heavily tegumented capsids are marked with arrows in panel b. Also present in panel a is a phage T4 virion, which was included because its tail provided an internal magnification standard. Bar, 100 nm. (c) Gallery of cores of nuclear B-capsids. The three left panels show such a capsid and the separated images of its surface shell and core. Bar, 50 nm. The next three panels show the cores of other capsids. The last two panels show an averaged image of the core and a radial density profile calculated by rotational averaging of this image. They disclose a double ring surrounding some central density. The tick mark on the x axis of the density profile denotes a radius of 50 nm.

Cytoplasmic B-capsids are less uniform in appearance (Fig. 2b). Many of them (40 to 50%) resemble nuclear B-capsids. The remainderhave additional material attached to their outer surface: of these,a subset of ~8% carry markedly greater amounts of this material(Fig. 2b, arrows). Consistent with its location on the outer surfaceof the capsid and the presence of specific tegument proteins inthis preparation (Fig. 1), we interpret this material as tegumentand view the three classes of particles as varying in the extentto which they have acquired or retained such proteins. We referto them as lightly, moderately, and heavily tegumented cytoplasmicB-capsids, respectively, noting that these are relative termsand that, in virions, the capsid may be still more heavily tegumented.Most of the heavily tegumented B-capsids (55 to 60%) had littleor no internal density: in contrast, only ~8% of the remainingcytoplasmic B-capsids were empty, a finding similar to the proportionof empty nuclear B-capsids (~9%).

To obtain unobstructed views of the inner shell, the coprojected surface shell was computationally erased from a set of particlesby subtracting reprojections of a three-dimensional density mapof the capsid (see below) that had been emptied by setting itsinternal densities to the background value. A gallery of coresis shown in Fig. 2c: some are more circularly symmetric than others,and it is likely that they represent cores in a relatively goodstate of preservation (see Discussion). The averaged core imageshows two closely spaced concentric rings and a central patchof density (Fig. 2c, rightmostpanels).

Nuclear B-capsids of SCMV and HSV-1 compared. To examine the structure of the nuclear B-capsid, we calculated a three-dimensional density map to a 2.2-nm resolution (Fig.3a and d). The molecular architecture of the capsid is largelyconserved between SCMV and other previously characterized herpesviruses,i.e., in the T=16 triangulation geometry; in the overall shapeof the large and elaborate capsomers, whose columnar protrusionsextend ~10 nm out from the contiguous "floor"; and in the presenceof triplexes at the threefold sites between capsomer protrusions.On the HSV-1 capsid, the 12-kDa VP26 (UL35) protein (20, 41)is present around the outer rims of the hexons but absent fromthe pentons (11, 65, 72, 73). We infer that this propertyalso is reproduced in SCMV because the protuberances around therims of its hexons are considerably larger than those on the pentons(cf. Fig. 3a and b and 6a). Thus, the additional outer part ofthe SCMV hexon protuberance represents a monomer of SCP (~8 kDa[32]), its counterpart to VP26 (see Fig. 6b).

View larger version (149K):
[in this window]
[in a new window]

FIG. 3. Reconstructed density map of nuclear B-capsids of SCMV at 2.2-nm resolution, viewed along an axis of twofold symmetry showing the outer surface (a) and the inner surface (d). Bar (d), 10 nm. To allow comparison with the HSV-1 capsid (at 2.4-nm resolution, reproduced from reference 17), corresponding features centered on the E-hexon, midway between two pentons, are compared in panels b and c and panels e and f: b and e, SCMV; c and f, HSV-1; b and c, outer surfaces; e and f, inner surfaces. Bar (b), 10 nm. On the outer surface, the orientations of the capsomer protrusions differ between SCMV and HSV-1 (cf. panels b and c). In principle, this might reflect an arbitrarily different assignment of handedness to the two T=16 density maps (handedness is a subtle feature in nonskewed icosahedral lattices, such as T=16). However, the relative handedness of the capsids was determined by maximizing the correlation between the two maps, and they match well in respect to the handedness on the inner surface (cf. panels e and f) and elsewhere. Thus, we consider that the differing orientations of their external protrusions is a genuine distinction, although the absolute handedness of either capsid has yet to be determined.

At a more detailed level, differences are apparent between the outer surfaces of the HSV-1 and SCMV capsomers (cf. Fig. 3band c), whereas the inner surfaces are almost superimposable (cf.Fig. 3e and f). The main structural distinctions relate to theouter parts of the respective hexon protrusions, which lie indifferent orientations relative to the surface lattice. Moreover,they have different shapes: in SCMV, unlike HSV-1, there are deepnotches between the protuberances around the outer rims of thecapsomer protrusions (cf. Fig. 3b and c), suggesting that thecorresponding portions of their major capsid proteins are foldeddifferently. Their respective triplexes also have somewhat differentshapes.

The SCMV capsid is slightly larger than the HSV-1 capsid, as assessed in terms of spherically averaged radial density profiles(Fig. 4). In outer radius, it is ~2% larger but the inner radiusis ~4% larger, the SCMV shell being slightly thinner. Both radialprofiles show three peaks in the surface shell, between ~50 and65 nm. For SCMV, the second peak is lower relative to the firstpeak than for HSV-1.

View larger version (29K):
[in this window]
[in a new window]

FIG. 4. Radial density profiles of SCMV capsids: nuclear B-capsids (red), lightly tegumented cytoplasmic B-capsids (blue), and heavily tegumented cytoplasmic B-capsids (green). Also shown for comparison (in black) is the profile of HSV-1 nuclear B-capsids (reproduced from reference 17). The curves were obtained by spherical averaging of the corresponding three-dimensional density maps. The inner part of these curves (r < 40 nm, relating to the core) becomes progressively noisier towards the lower radii, both because of sparser sampling and because some distorted cores were included in the calculation. An optimized rendition of this part of the profile, calculated from nuclear B-capsids with well-preserved cores (see Materials and Methods), is shown below (in gray) offset, relative to the other curves, for clarity.

Radial organization of nuclear and cytoplasmic B-capsids. The material adhering to heavily tegumented cytoplasmic B-capsids appears not to be arranged with perfect icosahedral symmetry,to judge by its irregular appearance. We found it more difficultto determine their orientations than for other capsids in thesame micrographs, presumably because of this material. Nevertheless,enough particles (79 in all) were solved to yield a well definedmap at 2.5-nm resolution. We also generated maps at a 2.2-nm resolutionfrom larger numbers of moderately and lightly tegumented B-capsids.

Averaged radial density profiles were calculated from these maps, and those of the lightly and heavily tegumented B-capsidsare compared in Fig. 4 with that of nuclear B-capsids. In theinner part of the capsid shell, i.e., between radii of ~48 and~58 nm, the curves of the lightly and heavily tegumented B-capsidsare superimposable and differ slightly in relative peak heightsfrom that of the nuclear B-capsid, which may reflect slight conformationaldifferences between them. From ~58 to ~65 nm, the profile of theheavily tegumented B-capsid overlies that of the lightly tegumentedB-capsid by a small margin, and both have more density in thisregion than the nuclear B-capsid. Between 65 and 70 nm, the additionalouter density of heavily tegumented B-capsids becomes moreevident.

SCMV B-capsids contain an inner shell, which lies between radii of ~20 and ~40 nm and is separated from the surface shellby a gap of ~10 nm (Fig. 4). In contrast, the internal proteinsof HSV-1 B-capsids, which are not regularly ordered in a shellbut are icosahedrally averaged in the reconstruction, registerno inner edge (cf. Fig. 4). At lower radii, these profiles becomeprogressively noisier but nevertheless reveal the following features.Their overall shapes are generally similar for all kinds of SCMVB-capsids, although the profile of heavily tegumented B-capsidsis ~50% lower, reflecting their higher proportion of empty capsids.The curves all show a minimum at a radius of ~28 nm and an outershoulder located between ~33 and ~40nm.

The inner part of the profile (i.e., at radii of <40 nm) is smeared because not all particles included in the reconstructionhave well-preserved cores. Some have lesions that suggest incipientdegeneration and other cores are off-centered (Fig. 2a). However,by selecting particles with round, seemingly well preserved coresand correcting for off-centering, we calculated an optimized averagedimage (Fig. 2c). After rotational averaging to obtain a projectionprofile, two density peaks are clearly resolved at radii of ~25and 30 nm, respectively (Fig. 2c, rightmost panel). From thiscurve, an average radial density profile was calculated (Fig.4, bottom curve), which shows more clearly the strong minimumbetween them at the 28-nmradius.

Visualization of capsid-tegument interactions. The outer surfaces of moderately and heavily tegumented cytoplasmic B-capsids are presented in stereo in Fig. 5a and b. Figure5c is a difference map calculated between the moderately tegumentedcytoplasmic B-capsid and the nuclear B-capsid. The two maps areat the same resolution (2.2 nm), and this difference map is intendedto highlight any additional components present on cytoplasmicB-capsids. Although there is some noise that we attribute mainlyto minor conformational differences between the respective shells,the most pronounced difference is the presence of additional densitycapping each subunit of major capsid protein. This density iscarrot-shaped, ~6 nm long by ~2.5 nm wide at its midpoint, andoriented with its long axis tangential to the capsid surface andits tapered end pointing in towards the symmetry axis of the capsomer(Fig. 6c; see also Fig. 5c, lower right quadrant). Similarly shapedfeatures overlie both the hexons and the pentons (see also Fig.8a). Presumably, they represent protein subunits, and we referto them as the capsomer-capping protein(s). Consistent resultswere obtained with a difference map calculated between lightlytegumented cytoplasmic B-capsids and nuclear B-capsids (data notshown).

View larger version (100K):
[in this window]
[in a new window]

FIG. 5. Stereo pairs presenting the outer surfaces of the moderately tegumented cytoplasmic B-capsid (a) and the heavily tegumented cytoplasmic B-capsid (b) of SCMV. Also shown are difference maps of the moderately tegumented cytoplasmic B-capsid minus the nuclear B-capsid (c) and the heavily tegumented cytoplasmic B-capsid minus the moderately tegumented cytoplasmic B-capsid (d). Because we wished to focus on components associated with the outer surface of the capsid, the internal density was set to zero in both maps to avoid distracting differences from the relatively noisy internal regions. Map c reveals the capsomer-capping tegument protein, and map d reveals the triplex-associated tegument protein. Bar (a), 10 nm.

We also calculated a difference map between the heavily and moderately tegumented cytoplasmic B-capsids (Fig. 5d) to accentuatecomponents that are present in higher occupancy on the former.The predominant features of this difference map are V-shaped densitiesextending from the triplexes. The tip of the V makes contact withthe triplex, and its legs are ~10 nm long and 2 to 2.5 nm thick.We infer that the two halves of the V represent two copies ofthe triplex-associatedprotein.

The molecular weights of these proteins were estimated from their apparent volumes, applying a partial specific volume typicalfor protein. We gauged the reliability of the method by usingit to measure the mass of a triplex in a density map of HSV-1capsid, contoured to contain 100% of the total mass as determinedby scanning transmission electron microscopy (43). The valueobtained was 130 kDa, ~8% higher than the theoretical value of119 kDa (one copy of VP19c plus two copies of VP23). In the sameway, the mass of the penton-capping protein was estimated fromthe SCMV density maps as 50 to 60 kDa and that of the triplex-associatedprotein as 100 to 120 kDa. We note that, notwithstanding our controlexperiment, such estimates may be biased downwards by substoichiometricoccupancy or localdisordering.

The outer surfaces of these capsids in the region around a penton are shown at higher magnification in Fig. 6. The nuclearB-capsid is shown in Fig. 6a, a diagram marking its salient featuresin Fig. 6b, and the moderately and heavily tegumented cytoplasmicB-capsids in Fig. 6c and d, respectively. The inner surfaces ofall three classes of cytoplasmic B-capsids are essentially identicalwhen depicted at the same resolution. As a representative, thatof the moderately tegumented cytoplasmic B-capsid (Fig. 6f) iscompared with that of the nuclear B-capsid (Fig. 6e). Minor differencesbetween them (cf. Fig. 6e and f) suggest that the surface shellsof nuclear and cytoplasmic B-capsids may be in slightly differentconformations.

View larger version (134K):
[in this window]
[in a new window]

FIG. 6. Peripentonal regions of the outer (a to d) and inner (e and f) surfaces of SCMV capsids. Panels: a, nuclear B-capsid; b, diagram indexing features of note in panel a, where SCP is the smallest capsid protein present on hexons (gray outer portion of protuberance on top of the hexon subunits) but not on pentons, where the corresponding protuberance is markedly smaller and rounder; c, moderately tegumented cytoplasmic capsid; d, heavily tegumented cytoplasmic capsid. Also shown are the inner surfaces of the nuclear B-capsid (e) and the moderately tegumented cytoplasmic B-capsid (f). Bar, 10 nm.

To visualize components that, although not stoichiometric, are present in sufficient quantity to be discernible in a reconstruction,it is informative to examine sections through the maps (Fig. 7).The core is visible in our maps of both the nuclear B-capsid (Fig.7a) and the moderately tegumented cytoplasmic B-capsid (Fig. 7b).The triplex-associated protein is faintly visible in the moderatelytegumented B-capsid (Fig. 7e), whereas in the heavily tegumentedB-capsid (Fig. 7f), it is as strongly represented as the capsidproteins, implying full occupancy. This protein is anchored onthe triplex, passes along the wall of the capsomer protrusion,makes contact with the capsomer-capping protein (see Fig. 6c and8a), and then extends out beyond the protrusions. In all threecytoplasmic B-capsids, the density associated with the capsomer-cappingprotein (Fig. 7h and i, arrows) is similar to that of the majorcapsid protein, suggesting full occupancy.

View larger version (155K):
[in this window]
[in a new window]

FIG. 7. Central sections (half-plane) through density maps of the nuclear B-capsid (a), moderately tegumented cytoplasmic B-capsid (b), and heavily tegumented cytoplasmic B-capsid (c) of SCMV. The plane of the 0.4-nm-thick section is perpendicular to an axis of twofold icosahedral symmetry and passes centrally through pentons (p), peripentonal hexons (h_p), edge hexons (h_E), and central hexons (h_c) (see Fig. 2 of reference 60 for nomenclature) and triplexes (T). The regions centered on the h_E hexon and the penton from all three maps are compared at higher magnification in panels d to i. The arrows in panels e and f indicate the additional density on cytoplasmic B-capsids, which is attributed to the triplex-associated tegument protein. This density is faint in panel e and strong in panel f. The arrows in panels h and i indicate the additional density attributed to the capsomer-capping protein (here, on the penton) on both kinds of cytoplasmic B-capsids. The difference in this density on either side of the penton occurs because the section plane passes centrally through this protein only on one side of the penton. The distribution of capsomer-capping protein subunits over the capsid surface is shown in Fig. 5c. Bars (a and d), 10 nm.

The components of the heavily tegumented cytoplasmic B-capsid, i.e., its capsid shell, the capsomer-capping protein, and thetriplex-associated protein, are distinguished by color codingin Fig. 8a. The apparent connectivity of the interactions thatlink them together is shown schematically in Fig. 8b.

View larger version (109K):
[in this window]
[in a new window]

FIG. 8. (a) Region surrounding the fivefold axis showing the interactions of the two major tegument proteins with the SCMV capsid. The capsomer-capping tegument protein is shown as blue, and the triplex-associated tegument protein is shown as red. The segmentation was achieved by removing noise from the two difference maps (Fig. 5c and d) and then recombining them with the nuclear B-capsid image. Bar, 10 nm. (b) Schematic summary of the interactions that link the tegument to the capsid. The capsomer-capping tegument protein (blue) binds to the major capsid protein on top of the capsomer protrusions. Two copies of the triplex-binding tegument protein (red) diverge from each triplex (the triplex is shown in panel b as a triangle). This elongated protein contacts the capsomer-capping protein (blue) on two different capsomers and then extend outwards. This protein may have an additional domain or domains that extend beyond the portions sketched in panel b, which are not well visualized in our density map (panels b and c) on account of flexibility or otherwise poor ordering.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

We have investigated the capsid structure of SCMV, viewed as a representative betaherpesvirus. To date, the only other herpesviruseswhose capsids have been characterized in comparable detail arethe alphaherpesviruses, EHV-1 (3) and HSV-1 (e.g., references17 and 73), and channel catfish virus (10), a distant andstill-uncategorized relative (19). The molecular architectureof the nuclear B-capsid of SCMV turned out to be quite similarto those already described, a finding consistent with its proteincomposition being conserved (25, 28). Nevertheless, severaldifferences came to light in the presentstudy.

Limited variability in capsid size among herpesviruses. Since CMVs have the largest genomes of all herpesviruses, one might expect corresponding adaptations in capsid structure.However, the average inner radius of SCMV (49.5 nm) is only slightlygreater than those of HSV-1 (47.2 nm) and channel catfish virus(45.9 nm), whose packing densities are quite similar (9). Withthe same packing density as HSV-1, the SCMV capsid would accommodatea genome of ~171 kbp. Although the SCMV genome has not yet beencompletely sequenced, estimates from restriction enzyme digestsindicate that its size is higher at ~209 kbp (33a). The additionalDNA could be accommodated by slightly tighter packing, i.e., reducingthe interduplex spacing of HSV-1 (9) by 7% would give a spacingof 2.57 nm, which remains reasonable for packaged viral DNA (cf.2.54 nm for bacteriophage T7 [15]). In summary, we expect thatother herpesvirus genomes are packed in much the same "liquidcrystalline" fashion as in HSV-1 (9), whereby substantial variationsin genome size may be accommodated by proportionately much smallerchanges in capsid dimensions and/or packingdensity.

The small core of isolated SCMV B-capsids. Most of these capsids contain an inner shell composed mainly of the assembly protein in its mature, proteolytically processedform (31, 69). Presumably, these structures were originallyassembled as procapsid scaffolds (64) and subsequently contractedupon proteolytic processing and maturation of the procapsid, intheir transition from large-cored to small-cored B-capsids (49,62). The large gap between the inner and outer shells (Fig.4) supports this explanation. Although isolated B-capsids of EHV-1(3) and HSV-1 (44) were found to contain irregular coagulatesof their assembly proteins, their appearance as small cores inthin sections of infected cells (see, for example, reference 47)implies that this material was originally organized like the innershell of SCMV B-capsids but became disordered duringisolation.

Domain structure of assembly protein. There is strong physical (3, 50) and biochemical (43) evidence that the small cores of herpesvirus B-capsids are composedprimarily of the scaffolding-assembly protein in its proteolyticallycleaved form. Accordingly, examination of the spherical smallcore of SCMV may yield some insight into the structure of thiskey morphogenic protein. We confine this discussion to its optimizedradial density profile (Fig. 4, lower curve), which describesthe distribution of mass along this molecule. The profile discloses,in addition to some material at the center, a shell that is ~16nm thick, with peaks separated by a minimum at a radius of ~28nm. Deferring interpretation of the material at the center, thisprofile implies that the 30-kDa assembly protein is an elongatedmolecule (~16 nm) and consists of two domains separated by a low-densitylinker.

The outer domain is presumably the C-terminal moiety, since the C terminus of the precursor should interact with the surfaceshell (7, 21, 36, 44, 45, 69, 71). We tentativelysuggest that the linker may be an $alpha$ -helical coiled coil, aboutfour heptads (4 nm) long, based on scanning the SCMV assemblyprotein sequence (68) with a coiled-coil detection algorithm(40) (unpublished results). Such a coiled coil has been reportedfor the assembly protein of HSV-1 (45), and we note that theradial profile of the inner shell of the HSV-1 procapsid alsoexhibits a pronounced minimum (cf. Fig. 6 of reference 64).

Variable tegumentation of cytoplasmic B-capsids. The origins of cytoplasmic B-capsids and their relationship to the export pathway of maturing virions are not clear. We obtainedthese capsids in significant amounts only at very late times afterinfection, when their appearance in the cytoplasm may reflectdeteriorating nuclear and/or cytoplasmic compartmentation. Weconsider it unlikely that they derive from infecting virions,since the majority retain assembly protein, which is absent fromvirions. However, about one-half of the heavily tegumented B-capsids(~5% of the total) are coreless, and it is not ruled out thatthey represent infecting virions that have discharged their genomes.Heavily tegumented cytoplasmic B-capsids may represent a moreadvanced stage of tegumentation or a subpopulation that fortuitouslyretained more of its tegument through the isolation procedure.Notwithstanding their origins or maturation prospects, cytoplasmicB-capsids afford the possibility of insight into capsid-tegumentinteractions.

Interactions between capsid and tegument. The three classes of cytoplasmic B-capsids were reconstructed separately. Comparing these reconstructions with each otherand with the nuclear B-capsid revealed two sites of tegument attachment.On all cytoplasmic B-capsids, each capsomer subunit is cappedwith an additional protein (Fig. 5c, 7h, and 7i), i.e., this proteinis approximately equimolar with the major capsid protein. Althoughthe proteins that overlie hexons and pentons, respectively, aresimilar in size and shape and binding site on the capsomer protrusions,the penton-associated protein may be slightly longer, and it isnot ruled out that more than one species is involved. Althoughthe smallest capsid protein (SCP) is present around the outerrim of hexons, the capsomer-capping protein(s) presumably bindsto the major capsid protein, since it is also present on pentons,which lack the SCP (cf. Fig. 6a toc).

The second protein that we have detected has a V-shaped structure, whose tip is anchored on a triplex and whose "legs" divergeoutwards. This protein makes contact with the capsomer-cappingprotein at the tips of neighboring capsomer protrusions, beforeit extends into the outer region of diffuse density (Fig. 5d and7f). This triplex-associated protein is faintly visible in themoderately tegumented B-capsid, reflecting low occupancy, andis strongly visible in the heavily tegumented B-capsid, reflectingnearly complete occupancy (cf. Fig. 7e and f). As noted above,it is likely to be a dimer, in which case it should be bound tothe minor capsid protein (the counterpart of VP23 of HSV-1 [43]),which is present in two copies per triplex (6). At full occupancy,there would be 640 copies of this protein percapsid.

Candidates for the capsid-binding tegument proteins. Current evidence does not allow conclusive identification of either protein. However, by correlating their molecular sizesand abundances, as estimated by electron microscopy and with correspondingdata from SDS-PAGE, we can identify possiblecandidates.

The triplex-associated protein M_r value was estimated to be 100,000 to 120,000, which tallies with BPP (~119,000). Its molarratio relative to the major capsid protein in this preparationwas approximated from the observed proportions of lightly, moderately,and heavily tegumented B-capsids, and its amount on each, as givenby its map density relative to that of the major capsid proteinand a stoichiometry of two copies per triplex. This calculationyielded a figure of ~0.15, which is in reasonable agreement withthe value obtained for BPP by quantitating the stained gel bands(i.e., 0.13). At full occupancy, the triplex-associated proteinwould have a molar ratio of 0.67 relative to the major capsidprotein, which is close to the value of 0.8 estimated for BPPin virions (37). These correlations suggest BPP as a plausiblecandidate for thisprotein.

We estimate the capsomer-capping protein(s) to be ~50 to 60 kDa and close to equimolar with the major capsid protein. CytoplasmicB-capsids contain proteins in this size range (cf. Fig. 1), butthe complexity and close spacing of the protein bands in thisregion of the gel precluded reliable quantitation. The only knowntegument proteins in this size range that are of appropriate abundancein virions are the matrix proteins, UM and LM (26, 37). UMhas been reported to be equimolar with the major capsid protein(25, 37), whereas LM has been found to vary considerably inamount among the different strains of CMV (38) and is not requiredfor virion assembly (55). These considerations may favor UMas a candidate. However, further data are required to test thishypothesis.

Binding of other tegument proteins. Our reconstructions assume icosahedral symmetry and thus reveal only the most highly ordered part of the tegument, the partin direct contact with the capsid shell. As such, these observationsrepresent only a first step towards an account of the molecularorganization of the tegument. Nevertheless, they imply that thecoupling of the SCMV tegument to its capsid is not confined topentons (66) but is instead distributed all over the capsidsurface.

Each copy of the major capsid protein, in hexons and pentons alike, is capped with an additional protein. If this capsomer-cappingprotein is a single species, it differs in this respect from theSCP which binds only to hexons (cf. Fig. 6a) as a consequenceof differences between the penton and hexon conformations of themajor capsid protein (70). We have conjectured (70) that theabsence of SCP from pentons may confer the advantage of diversifyingthe binding sites presented on the capsid surface, which couldfacilitate the binding of different tegument proteins. However,if the same capsomer-capping protein binds to both hexons andpentons, this opportunity is not exploited in tegumentation, atleast, for SCMV. It may, however, be relevant to interactionsin which the capsid engages at other stages of the replicationcycle (cf. references 5, 34, 35, 46, and 58).

A diffuse outer halo of density is seen in the maps of moderately and heavily tegumented B-capsids (Fig. 2b, Fig. 4, and Fig.7b and c), indicating that some proteins are present in this region,albeit in a disordered state. The triplex-associated protein extendsinto this region, where it may serve as a platform for other tegumentcomponents. However, the mechanisms whereby they are selectedand bound, and how they may function in envelopment or in otherviral functions, remain to beaddressed.

	ACKNOWLEDGMENTS

We thank T. Baker and J. Conway for software, D. Belnap for helpful discussions, and S. Butcher for dialog on CMVstructure.

This work was supported in part by USPHS grant AI13718 to W.G.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Structural Biology, NIAMS, Bldg. 6, Rm. B2-34, 6 Center Dr., MSC 2717,National Institutes of Health, Bethesda, MD 20892-2717. Phone:(301) 496-0132. Fax: (301) 480-7629. E-mail: Alasdair_Steven{at}nih.gov.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

1. Baker, T. S., and R. H. Cheng. 1996. A model-based approach for determining orientations of biological macromolecules imaged by cryoelectron microscopy. J. Struct. Biol. 116:120-130[Medline].

2. Baker, T. S., J. Drak, and M. Bina. 1988. Reconstruction of the three-dimensional structure of simian virus 40 and visualization of the chromatin core. Proc. Natl. Acad. Sci. USA 85:422-426[Abstract/Free Full Text].

3. Baker, T. S., W. W. Newcomb, F. P. Booy, J. C. Brown, and A. C. Steven. 1990. Three-dimensional structures of maturable and abortive capsids of equine herpesvirus 1 from cryoelectron microscopy. J. Virol. 64:563-573[Abstract/Free Full Text].

4. Bankier, A. T., S. Beck, R. Bohni, C. M. Brown, R. Cerny, M. S. Chee, C. A. Hutchison, T. Kouzarides, J. A. Martignetti, and E. Preddie. 1991. The DNA sequence of the human cytomegalovirus genome. DNA Seq. 2:1-12[Medline].

5. Batterson, W., D. Furlong, and B. Roizman. 1983. Molecular genetics of herpes simplex virus. VIII. Further characterization of a temperature-sensitive mutant defective in release of viral DNA and in other stages of the viral replicative cycle. J. Virol. 45:397-407[Abstract/Free Full Text].

6. Baxter, M., and W. Gibson. 1997. The putative human cytomegalovirus triplex proteins, minor capsid protein (mCP) and mCP-binding protein (mC-BP), form a heterotrimeric complex that localizes to the cell nucleus in the absence of other viral proteins. 22nd International Herpesvirus Workshop, La Jolla, Calif .

7. Beaudet-Miller, M., R. Zhang, J. Durkin, W. Gibson, A. D. Kwong, and Z. Hong. 1996. Viral specific interaction between the human cytomegalovirus major capsid protein and the C terminus of the precursor assembly protein. J. Virol. 70:8081-8088[Abstract].

8. Black, L. W., M. K. Showe, and A. C. Steven. 1994. Morphogenesis of the T4 head, p. 218-258. In J. Karam (ed.), Molecular biology of bacteriophage T4. American Society for Microbiology, Washington, D.C.

9. Booy, F. P., W. W. Newcomb, B. L. Trus, J. C. Brown, T. S. Baker, and A. C. Steven. 1991. Liquid-crystalline, phage-like, packing of encapsidated DNA in herpes simplex virus. Cell 64:1007-1015[Medline].

10. Booy, F. P., B. L. Trus, A. J. Davison, and A. C. Steven. 1996. The capsid architecture of channel catfish virus, an evolutionarily distant herpesvirus, is largely conserved in the absence of discernible sequence homology with herpes simplex virus. Virology 215:134-141[Medline].

11. Booy, F. P., B. L. Trus, W. W. Newcomb, J. C. Brown, J. F. Conway, and A. C. Steven. 1994. Finding a needle in a haystack: detection of a small protein (the 12 kDa VP26) in a large complex (the 200 MDa capsid of herpes simplex virus). Proc. Natl. Acad. Sci. USA 91:5652-5656[Abstract/Free Full Text].

12. Brown, J. H., C. Cohen, and D. A. Parry. 1996. Heptad breaks in alpha-helical coiled coils: stutters and stammers. Proteins 26:134-145[Medline].

13. Campadelli-Fiume, G., F. Farabegoli, S. Di Gaeta, and B. Roizman. 1991. Origin of unenveloped capsids in the cytoplasm of cells infected with herpes simplex virus 1. J. Virol. 65:1589-1595[Abstract/Free Full Text].

14. Casjens, S., and R. Hendrix. 1988. Control mechanisms in dsDNA bacteriophage assembly, p. 15-91. In R. Calendar (ed.), The bacteriophages. Plenum Publishing Corp., New York, N.Y.

15. Cerritelli, M. E., N. Cheng, A. H. Rosenberg, C. E. McPherson, F. P. Booy, and A. C. Steven. 1997. Encapsidated conformation of bacteriophage T7 DNA. Cell 91:271-280[Medline].

16. Conway, J. F., R. L. Duda, N. Cheng, R. W. Hendrix, and A. C. Steven. 1995. Proteolytic and conformational control of virus capsid maturation: the bacteriophage HK97 system. J. Mol. Biol. 253:86-99[Medline].

17. Conway, J. F., B. L. Trus, F. P. Booy, W. W. Newcomb, J. C. Brown, and A. C. Steven. 1996. Visualization of three-dimensional density maps reconstructed from cryoelectron micrographs of viral capsids. J. Struct. Biol. 116:200-208[Medline].

18. Davison, A. 1998. Herpesvirus genes. Rev. Med. Virol. 3:237-244.

19. Davison, A. J. 1992. Channel catfish virus: a new type of herpesvirus. Virology 186:9-14[Medline].

20. Davison, M. D., F. J. Rixon, and A. J. Davison. 1992. Identification of genes encoding two capsid proteins (VP24 and VP26) of herpes simplex virus type 1. J. Gen. Virol. 73:2709-2713[Abstract/Free Full Text].

21. Desai, P., and S. Person. 1996. Molecular interactions between the HSV-1 capsid proteins as measured by the yeast two-hybrid system. Virology 220:516-521[Medline].

22. Fuller, S. D. 1987. The T=4 envelope of Sindbis virus is organized by interactions with a complementary T=3 capsid. Cell 48:923-934[Medline].

23. Fuller, S. D., S. J. Butcher, R. H. Cheng, and T. S. Baker. 1996. Three-dimensional reconstruction of icosahedral particles $---$ the uncommon line. J. Struct. Biol. 116:48-55[Medline].

24. Gibson, W. 1981. Structural and nonstructural proteins of strain Colburn cytomegalovirus. Virology 111:516-537[Medline].

25. Gibson, W. 1983. Protein counterparts of human and simian cytomegaloviruses. Virology 128:391-406[Medline].

26. Gibson, W. 1991. Cytomegalovirus protein structure and function. Elsevier Science Publishers B. V., Amsterdam, The Netherlands.

27. Gibson, W. 1993. Molecular biology of human cytomegalovirus. Springer-Verlag, New York, N.Y.

28. Gibson, W. 1996. Structure and assembly of the virion. Intervirology 39:389-400[Medline].

29. Gibson, W., and B. Roizman. 1972. Proteins specified by herpes simplex virus. VIII. Characterization and composition of multiple capsid forms of subtypes 1 and 2. J. Virol. 10:1044-1052[Abstract/Free Full Text].

30. Gibson, W., R. van Breemen, A. Fields, R. LaFemina, and A. Irmiere. 1984. D,L-alpha-difluoromethylornithine inhibits human cytomegalovirus replication. J. Virol. 50:145-154[Abstract/Free Full Text].

31. Gibson, W., A. I. Marcy, J. C. Comolli, and J. Lee. 1990. Identification of precursor to cytomegalovirus capsid assembly protein and evidence that processing results in loss of its carboxy-terminal end. J. Virol. 64:1241-1249[Abstract/Free Full Text].

32. Gibson, W., K. S. Clopper, W. J. Britt, and M. K. Baxter. 1996. Human cytomegalovirus (HCMV) smallest capsid protein identified as product of short open reading frame located between HCMV UL48 and UL49. J. Virol. 70:5680-5683[Abstract/Free Full Text].

33. Gibson, W., M. K. Baxter, and K. S. Clopper. 1996. Cytomegalovirus "missing" capsid protein identified as heat-aggregable product of human cytomegalovirus UL46. J. Virol. 70:7454-7461[Abstract].

33a. Hayward, G. Personal communication.

34. Hensel, G., H. Meyer, S. Gärtner, G. Brand, and H. F. Kern. 1995. Nuclear localization of the human cytomegalovirus protein pp150 (ppUL32). J. Gen. Virol. 76:1591-1601[Abstract/Free Full Text].

35. Hensel, G. M., H. H. Meyer, I. Buchmann, D. Pommerehne, S. Schmolke, B. Plachter, K. Radsak, S. Gärtner, G. Brand, and H. F. Kern. 1996. Intracellular localization and expression of the human cytomegalovirus matrix phosphoprotein pp71 (ppUL82): evidence for its translocation into the nucleus. J. Gen. Virol. 77:3087-3097[Abstract/Free Full Text].

36. Hong, Z., M. Beaudet-Miller, J. Burkin, R. Zhang, and A. D. Kwong. 1996. Identification of a minimal hydrophobic domain in the herpes simplex virus type 1 scaffolding protein which is required for interaction with the major capsid protein. J. Virol. 70:533-540[Abstract].

37. Irmiere, A., and W. Gibson. 1983. Isolation and characterization of a noninfectious virion-like particle released from cells infected with human strains of cytomegalovirus. Virology 130:118-133[Medline].

38. Jahn, G., B.-C. Scholl, B. Traupe, and B. Fleckenstein. 1987. The two major structural phosphoproteins (pp65 and pp150) of human cytomegalovirus and their antigenic properties. J. Gen. Virol. 68:1327-1337[Abstract/Free Full Text].

39. Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].

40. Lupas, A., M. Van Dyke, and J. Stock. 1991. Predicting coiled coils from protein sequences. Science 252:1162-1164[Medline].

41. McNabb, D. S., and R. J. Courtney. 1994. Identification and characterization of the herpes simplex virus type 1 virion protein encoded by the UL35 open reading frame. J. Virol. 66:2653-2663[Abstract/Free Full Text].

42. Newcomb, W. W., F. L. Homa, F. P. Booy, D. R. Thomsen, B. L. Trus, A. C. Steven, J. V. Spencer, and J. C. Brown. 1996. Assembly of the herpes simplex virus capsid: characterization of intermediates observed during cell-free capsid formation. J. Mol. Biol. 263:432-446[Medline].

43. Newcomb, W. W., B. L. Trus, F. P. Booy, A. C. Steven, J. S. Wall, and J. C. Brown. 1993. Structure of the herpes simplex virus capsid: molecular composition of the pentons and triplexes. J. Mol. Biol. 232:499-511[Medline].

44. Oien, N. L., D. R. Thomsen, M. W. Wathen, W. W. Newcomb, J. C. Brown, and F. L. Homa. 1997. Assembly of herpes simplex virus capsids using the human cytomegalovirus scaffold protein: critical role of the C terminus. J. Virol. 71:1281-1291[Abstract].

45. Pelletier, A., F. Do, J. J. Brisebois, L. Lagace, and M. G. Cordingley. 1997. Self-association of herpes simplex virus type 1 ICP35 is via coiled-coil interactions and promotes stable interaction with the major capsid protein. J. Virol. 71:5197-5208[Abstract].

46. Penfold, M. E., P. Armati, and A. L. Cunningham. 1994. Axonal transport of herpes simplex virions to epidermal cells: evidence for a specialized mode of virus transport and assembly. Proc. Natl. Acad. Sci. USA 91:6529-6533[Abstract/Free Full Text].

47. Preston, V. G., J. A. Coates, and F. J. Rixon. 1983. Identification and characterization of a herpes simplex virus gene product required for encapsidation of virus DNA. J. Virol. 45:1056-1064[Abstract/Free Full Text].

48. Preston, V. G., F. J. Rixon, I. M. McDougall, M. McGregor, and M. F. Alkobaisi. 1992. Processing of the herpes simplex virus assembly protein-icp35 near its carboxy terminal end requires the product of the whole of the ul26 reading frame. Virology 186:87-98[Medline].

49. Rixon, F. J. 1993. Structure and assembly of herpesviruses. Semin. Virol. 4:135-144.

50. Rixon, F. J., A. M. Cross, C. Addison, and V. G. Preston. 1988. The products of herpes simplex virus type 1 gene UL26 which are involved in DNA packaging are strongly associated with empty but not with full capsids. J. Gen. Virol. 69:2879-2891[Abstract/Free Full Text].

51. Roffman, E., J. P. Albert, J. P. Goff, and N. Frenkel. 1990. Putative site for the acquisition of human herpesvirus 6 virion tegument. J. Virol. 64:6308-6313[Abstract/Free Full Text].

52. Roizman, B. 1996. Herpesviridae, p. 2221-2230. In B. N. Fields, and D. M. Knipe (ed.), Fields virology. Lippincott-Raven Publishers, Philadelphia, Pa.

53. Roizman, B., and D. Furlong. 1974. The replication of herpes viruses, p. 229-403. In H. Fraenkel-Conrat, and R. R. Wagner (ed.), Comprehensive virology. Plenum Press, New York, N.Y.

54. Schagger, H., and G. Von Jagow. 1987. Tricine-sodium dodecyl sulfate-polyacrylamide gel electrophoresis for the separation of proteins in the range from 1 to 100 kDa. Anal. Biochem. 166:368-379[Medline].

55. Schmolke, S., H. G. Kern, P. Drescher, G. Jahn, and B. Plachter. 1995. The dominant phosphoprotein pp65 of human cytomegalovirus. Virus Res. 69:5959-5968.

56. Sherman, G., and S. L. Bachenheimer. 1988. Characterization of intranuclear capsids made by morphogenic mutants of HSV-1. Virology 163:471-480[Medline].

57. Smith, J. D., and E. Harven. 1974. Herpes simplex virus and human cytomegalovirus replication in WI-38 cells. II. An ultrastructural study of viral penetration. J. Virol. 14:945-956[Abstract/Free Full Text].

58. Sodeik, B., M. W. Ebersold, and A. Helenius. 1997. Microtubule-mediated transport of incoming herpes simplex virus 1 capsids to the nucleus. J. Cell Biol. 136:1007-1021[Abstract/Free Full Text].

59. Spencer, J. V., W. W. Newcomb, D. R. Thomsen, F. L. Homa, and J. C. Brown. 1998. Assembly of the herpes simplex virus capsid: preformed triplexes bind to the nascent capsid. J. Virol. 72:3944-3951[Abstract/Free Full Text].

60. Steven, A. C., C. R. Roberts, J. Hay, M. E. Bisher, T. Pun, and B. L. Trus. 1986. Hexavalent capsomers of herpes simplex virus type 2: symmetry, shape, dimensions, and oligomeric status. J. Virol. 57:578-584[Abstract/Free Full Text].

61. Steven, A. C., J. F. Hainfeld, B. L. Trus, P. M. Steinert, and J. S. Wall. 1984. Radial distributions of density within macromolecular complexes determined from dark-field electron micrographs. Proc. Natl. Acad. Sci. USA 81:6363-6367[Abstract/Free Full Text].

62. Steven, A. C., and P. G. Spear. 1997. Herpesvirus capsid assembly and envelopment, p. 312-351. In W. Chiu, R. M. Burnett, and R. L. Garcea (ed.), Structural biology of viruses. Oxford University Press, New York, N.Y.

63. Tooze, J., M. Hollinshead, K. Reis, and H. Kern. 1993. Progeny vaccinia and human cytomegalovirus particles utilize early endosomal cisternae for their envelopes. Eur. J. Cell Biol. 60:163-178[Medline].

64. Trus, B. L., F. P. Booy, W. W. Newcomb, J. C. Brown, F. L. Homa, D. R. Thomsen, and A. C. Steven. 1996. The herpes simplex virus procapsid: structure, conformational changes upon maturation, and roles of the triplex proteins VP19c and VP23 in assembly. J. Mol. Biol. 263:447-462[Medline].

65. Trus, B. L., F. L. Homa, F. P. Booy, W. W. Newcomb, D. R. Thomsen, N. Cheng, J. C. Brown, and A. C. Steven. 1995. Herpes simplex virus capsids assembled in insect cells infected with recombinant baculoviruses: structural authenticity and localization of VP26. J. Virol. 69:7362-7366[Abstract].

66. Vernon, S. K., W. C. Lawrence, C. A. Long, B. A. Rubin, and J. B. Sheffield. 1982. Morphological components of herpesvirus. IV. Ultrastructural features of the envelope and tegument. J. Ultrastruct. Res. 81:163-171[Medline].

67. Weiner, D., and W. Gibson. 1983. Phosphorylation, maturational processing, and relatedness of strain Colburn matrix proteins. Virology 129:155-169[Medline].

68. Welch, A. R., L. M. McNally, and W. Gibson. 1991. Cytomegalovirus assembly protein nested gene family: four 3'-coterminal transcripts encode four in-frame, overlapping proteins. J. Virol. 65:4091-4100[Abstract/Free Full Text].

69. Welch, A. R., A. S. Woods, L. M. McNally, R. J. Cotter, and W. Gibson. 1995. A herpesvirus maturational protease, assemblin: identification of its gene, putative active site domain, and cleavage site. Proc. Natl. Acad. Sci. USA 88:10792-10796[Abstract/Free Full Text].

70. Wingfield, P. T., S. J. Stahl, D. R. Thomsen, F. L. Homa, F. P. Booy, B. L. Trus, and A. C. Steven. 1997. Hexon-only binding of VP26 reflects differences between the hexon and penton conformations of VP5, the major capsid protein of herpes simplex virus. J. Virol. 71:8955-8961[Abstract].

71. Wood, L. J., M. K. Baxter, S. M. Plafker, and W. Gibson. 1997. Human cytomegalovirus capsid assembly protein precursor (pUL80.5) interacts with itself and with the major capsid protein (pUL86) through two different domains. J. Virol. 71:179-190[Abstract].

72. Zhou, Z. H., B. V. V. Prasad, J. Jakana, F. J. Rixon, and W. Chiu. 1994. Protein subunit structures in the herpes simplex virus capsid determined from 400-kV spot-scan electron cryomicroscopy. J. Mol. Biol. 242:456-469[Medline].

73. Zhou, Z. H., J. He, J. Jakana, J. D. Tatman, F. J. Rixon, and W. Chiu. 1995. Assembly of VP26 in herpes simplex virus-1 inferred from structures of wild-type and recombinant capsids. Nat. Struct. Biol. 2:1026-1030[Medline].

Journal of Virology, March 1999, p. 2181-2192, Vol. 73, No. 3
0022-538X/99/$00.00+0

This article has been cited by other articles:

Seo, J.-Y., Britt, W. J. (2008). Multimerization of Tegument Protein pp28 within the Assembly Compartment Is Required for Cytoplasmic Envelopment of Human Cytomegalovirus. J. Virol. 82: 6272-6287 [Abstract] [Full Text]
Kalejta, R. F. (2008). Tegument Proteins of Human Cytomegalovirus. Microbiol. Mol. Biol. Rev. 72: 249-265 [Abstract] [Full Text]
Krautwald, M., Maresch, C., Klupp, B. G., Fuchs, W., Mettenleiter, T. C. (2008). Deletion or green fluorescent protein tagging of the pUL35 capsid component of pseudorabies virus impairs virus replication in cell culture and neuroinvasion in mice. J. Gen. Virol. 89: 1346-1351 [Abstract] [Full Text]
Brignole, E. J., Gibson, W. (2007). Enzymatic Activities of Human Cytomegalovirus Maturational Protease Assemblin and Its Precursor (pPR, pUL80a): Maximal Activity of pPR Requires Self-Interaction through Its Scaffolding Domain. J. Virol. 81: 4091-4103 [Abstract] [Full Text]
Loveland, A. N., Nguyen, N. L., Brignole, E. J., Gibson, W. (2007). The Amino-Conserved Domain of Human Cytomegalovirus UL80a Proteins Is Required for Key Interactions during Early Stages of Capsid Formation and Virus Production. J. Virol. 81: 620-628 [Abstract] [Full Text]
AuCoin, D. P., Smith, G. B., Meiering, C. D., Mocarski, E. S. (2006). Betaherpesvirus-Conserved Cytomegalovirus Tegument Protein ppUL32 (pp150) Controls Cytoplasmic Events during Virion Maturation.. J. Virol. 80: 8199-8210 [Abstract] [Full Text]
Seo, J.-Y., Britt, W. J. (2006). Sequence Requirements for Localization of Human Cytomegalovirus Tegument Protein pp28 to the Virus Assembly Compartment and for Assembly of Infectious Virus

1.	Baker, T. S., and R. H. Cheng. 1996. A model-based approach for determining orientations of biological macromolecules imaged by cryoelectron microscopy. J. Struct. Biol. 116:120-130[Medline].
2.	Baker, T. S., J. Drak, and M. Bina. 1988. Reconstruction of the three-dimensional structure of simian virus 40 and visualization of the chromatin core. Proc. Natl. Acad. Sci. USA 85:422-426[Abstract/Free Full Text].
3.	Baker, T. S., W. W. Newcomb, F. P. Booy, J. C. Brown, and A. C. Steven. 1990. Three-dimensional structures of maturable and abortive capsids of equine herpesvirus 1 from cryoelectron microscopy. J. Virol. 64:563-573[Abstract/Free Full Text].
4.	Bankier, A. T., S. Beck, R. Bohni, C. M. Brown, R. Cerny, M. S. Chee, C. A. Hutchison, T. Kouzarides, J. A. Martignetti, and E. Preddie. 1991. The DNA sequence of the human cytomegalovirus genome. DNA Seq. 2:1-12[Medline].
5.	Batterson, W., D. Furlong, and B. Roizman. 1983. Molecular genetics of herpes simplex virus. VIII. Further characterization of a temperature-sensitive mutant defective in release of viral DNA and in other stages of the viral replicative cycle. J. Virol. 45:397-407[Abstract/Free Full Text].
6.	Baxter, M., and W. Gibson. 1997. The putative human cytomegalovirus triplex proteins, minor capsid protein (mCP) and mCP-binding protein (mC-BP), form a heterotrimeric complex that localizes to the cell nucleus in the absence of other viral proteins. 22nd International Herpesvirus Workshop, La Jolla, Calif .
7.	Beaudet-Miller, M., R. Zhang, J. Durkin, W. Gibson, A. D. Kwong, and Z. Hong. 1996. Viral specific interaction between the human cytomegalovirus major capsid protein and the C terminus of the precursor assembly protein. J. Virol. 70:8081-8088[Abstract].
8.	Black, L. W., M. K. Showe, and A. C. Steven. 1994. Morphogenesis of the T4 head, p. 218-258. In J. Karam (ed.), Molecular biology of bacteriophage T4. American Society for Microbiology, Washington, D.C.
9.	Booy, F. P., W. W. Newcomb, B. L. Trus, J. C. Brown, T. S. Baker, and A. C. Steven. 1991. Liquid-crystalline, phage-like, packing of encapsidated DNA in herpes simplex virus. Cell 64:1007-1015[Medline].
10.	Booy, F. P., B. L. Trus, A. J. Davison, and A. C. Steven. 1996. The capsid architecture of channel catfish virus, an evolutionarily distant herpesvirus, is largely conserved in the absence of discernible sequence homology with herpes simplex virus. Virology 215:134-141[Medline].
11.	Booy, F. P., B. L. Trus, W. W. Newcomb, J. C. Brown, J. F. Conway, and A. C. Steven. 1994. Finding a needle in a haystack: detection of a small protein (the 12 kDa VP26) in a large complex (the 200 MDa capsid of herpes simplex virus). Proc. Natl. Acad. Sci. USA 91:5652-5656[Abstract/Free Full Text].
12.	Brown, J. H., C. Cohen, and D. A. Parry. 1996. Heptad breaks in alpha-helical coiled coils: stutters and stammers. Proteins 26:134-145[Medline].
13.	Campadelli-Fiume, G., F. Farabegoli, S. Di Gaeta, and B. Roizman. 1991. Origin of unenveloped capsids in the cytoplasm of cells infected with herpes simplex virus 1. J. Virol. 65:1589-1595[Abstract/Free Full Text].
14.	Casjens, S., and R. Hendrix. 1988. Control mechanisms in dsDNA bacteriophage assembly, p. 15-91. In R. Calendar (ed.), The bacteriophages. Plenum Publishing Corp., New York, N.Y.
15.	Cerritelli, M. E., N. Cheng, A. H. Rosenberg, C. E. McPherson, F. P. Booy, and A. C. Steven. 1997. Encapsidated conformation of bacteriophage T7 DNA. Cell 91:271-280[Medline].
16.	Conway, J. F., R. L. Duda, N. Cheng, R. W. Hendrix, and A. C. Steven. 1995. Proteolytic and conformational control of virus capsid maturation: the bacteriophage HK97 system. J. Mol. Biol. 253:86-99[Medline].
17.	Conway, J. F., B. L. Trus, F. P. Booy, W. W. Newcomb, J. C. Brown, and A. C. Steven. 1996. Visualization of three-dimensional density maps reconstructed from cryoelectron micrographs of viral capsids. J. Struct. Biol. 116:200-208[Medline].
18.	Davison, A. 1998. Herpesvirus genes. Rev. Med. Virol. 3:237-244.
19.	Davison, A. J. 1992. Channel catfish virus: a new type of herpesvirus. Virology 186:9-14[Medline].
20.	Davison, M. D., F. J. Rixon, and A. J. Davison. 1992. Identification of genes encoding two capsid proteins (VP24 and VP26) of herpes simplex virus type 1. J. Gen. Virol. 73:2709-2713[Abstract/Free Full Text].
21.	Desai, P., and S. Person. 1996. Molecular interactions between the HSV-1 capsid proteins as measured by the yeast two-hybrid system. Virology 220:516-521[Medline].
22.	Fuller, S. D. 1987. The T=4 envelope of Sindbis virus is organized by interactions with a complementary T=3 capsid. Cell 48:923-934[Medline].
23.	Fuller, S. D., S. J. Butcher, R. H. Cheng, and T. S. Baker. 1996. Three-dimensional reconstruction of icosahedral particles $---$ the uncommon line. J. Struct. Biol. 116:48-55[Medline].
24.	Gibson, W. 1981. Structural and nonstructural proteins of strain Colburn cytomegalovirus. Virology 111:516-537[Medline].
25.	Gibson, W. 1983. Protein counterparts of human and simian cytomegaloviruses. Virology 128:391-406[Medline].
26.	Gibson, W. 1991. Cytomegalovirus protein structure and function. Elsevier Science Publishers B. V., Amsterdam, The Netherlands.
27.	Gibson, W. 1993. Molecular biology of human cytomegalovirus. Springer-Verlag, New York, N.Y.
28.	Gibson, W. 1996. Structure and assembly of the virion. Intervirology 39:389-400[Medline].
29.	Gibson, W., and B. Roizman. 1972. Proteins specified by herpes simplex virus. VIII. Characterization and composition of multiple capsid forms of subtypes 1 and 2. J. Virol. 10:1044-1052[Abstract/Free Full Text].
30.	Gibson, W., R. van Breemen, A. Fields, R. LaFemina, and A. Irmiere. 1984. D,L-alpha-difluoromethylornithine inhibits human cytomegalovirus replication. J. Virol. 50:145-154[Abstract/Free Full Text].
31.	Gibson, W., A. I. Marcy, J. C. Comolli, and J. Lee. 1990. Identification of precursor to cytomegalovirus capsid assembly protein and evidence that processing results in loss of its carboxy-terminal end. J. Virol. 64:1241-1249[Abstract/Free Full Text].
32.	Gibson, W., K. S. Clopper, W. J. Britt, and M. K. Baxter. 1996. Human cytomegalovirus (HCMV) smallest capsid protein identified as product of short open reading frame located between HCMV UL48 and UL49. J. Virol. 70:5680-5683[Abstract/Free Full Text].
33.	Gibson, W., M. K. Baxter, and K. S. Clopper. 1996. Cytomegalovirus "missing" capsid protein identified as heat-aggregable product of human cytomegalovirus UL46. J. Virol. 70:7454-7461[Abstract].
33a.	Hayward, G. Personal communication.
34.	Hensel, G., H. Meyer, S. Gärtner, G. Brand, and H. F. Kern. 1995. Nuclear localization of the human cytomegalovirus protein pp150 (ppUL32). J. Gen. Virol. 76:1591-1601[Abstract/Free Full Text].
35.	Hensel, G. M., H. H. Meyer, I. Buchmann, D. Pommerehne, S. Schmolke, B. Plachter, K. Radsak, S. Gärtner, G. Brand, and H. F. Kern. 1996. Intracellular localization and expression of the human cytomegalovirus matrix phosphoprotein pp71 (ppUL82): evidence for its translocation into the nucleus. J. Gen. Virol. 77:3087-3097[Abstract/Free Full Text].
36.	Hong, Z., M. Beaudet-Miller, J. Burkin, R. Zhang, and A. D. Kwong. 1996. Identification of a minimal hydrophobic domain in the herpes simplex virus type 1 scaffolding protein which is required for interaction with the major capsid protein. J. Virol. 70:533-540[Abstract].
37.	Irmiere, A., and W. Gibson. 1983. Isolation and characterization of a noninfectious virion-like particle released from cells infected with human strains of cytomegalovirus. Virology 130:118-133[Medline].
38.	Jahn, G., B.-C. Scholl, B. Traupe, and B. Fleckenstein. 1987. The two major structural phosphoproteins (pp65 and pp150) of human cytomegalovirus and their antigenic properties. J. Gen. Virol. 68:1327-1337[Abstract/Free Full Text].
39.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].
40.	Lupas, A., M. Van Dyke, and J. Stock. 1991. Predicting coiled coils from protein sequences. Science 252:1162-1164[Medline].
41.	McNabb, D. S., and R. J. Courtney. 1994. Identification and characterization of the herpes simplex virus type 1 virion protein encoded by the UL35 open reading frame. J. Virol. 66:2653-2663[Abstract/Free Full Text].
42.	Newcomb, W. W., F. L. Homa, F. P. Booy, D. R. Thomsen, B. L. Trus, A. C. Steven, J. V. Spencer, and J. C. Brown. 1996. Assembly of the herpes simplex virus capsid: characterization of intermediates observed during cell-free capsid formation. J. Mol. Biol. 263:432-446[Medline].
43.	Newcomb, W. W., B. L. Trus, F. P. Booy, A. C. Steven, J. S. Wall, and J. C. Brown. 1993. Structure of the herpes simplex virus capsid: molecular composition of the pentons and triplexes. J. Mol. Biol. 232:499-511[Medline].
44.	Oien, N. L., D. R. Thomsen, M. W. Wathen, W. W. Newcomb, J. C. Brown, and F. L. Homa. 1997. Assembly of herpes simplex virus capsids using the human cytomegalovirus scaffold protein: critical role of the C terminus. J. Virol. 71:1281-1291[Abstract].
45.	Pelletier, A., F. Do, J. J. Brisebois, L. Lagace, and M. G. Cordingley. 1997. Self-association of herpes simplex virus type 1 ICP35 is via coiled-coil interactions and promotes stable interaction with the major capsid protein. J. Virol. 71:5197-5208[Abstract].
46.	Penfold, M. E., P. Armati, and A. L. Cunningham. 1994. Axonal transport of herpes simplex virions to epidermal cells: evidence for a specialized mode of virus transport and assembly. Proc. Natl. Acad. Sci. USA 91:6529-6533[Abstract/Free Full Text].
47.	Preston, V. G., J. A. Coates, and F. J. Rixon. 1983. Identification and characterization of a herpes simplex virus gene product required for encapsidation of virus DNA. J. Virol. 45:1056-1064[Abstract/Free Full Text].
48.	Preston, V. G., F. J. Rixon, I. M. McDougall, M. McGregor, and M. F. Alkobaisi. 1992. Processing of the herpes simplex virus assembly protein-icp35 near its carboxy terminal end requires the product of the whole of the ul26 reading frame. Virology 186:87-98[Medline].
49.	Rixon, F. J. 1993. Structure and assembly of herpesviruses. Semin. Virol. 4:135-144.
50.	Rixon, F. J., A. M. Cross, C. Addison, and V. G. Preston. 1988. The products of herpes simplex virus type 1 gene UL26 which are involved in DNA packaging are strongly associated with empty but not with full capsids. J. Gen. Virol. 69:2879-2891[Abstract/Free Full Text].
51.	Roffman, E., J. P. Albert, J. P. Goff, and N. Frenkel. 1990. Putative site for the acquisition of human herpesvirus 6 virion tegument. J. Virol. 64:6308-6313[Abstract/Free Full Text].
52.	Roizman, B. 1996. Herpesviridae, p. 2221-2230. In B. N. Fields, and D. M. Knipe (ed.), Fields virology. Lippincott-Raven Publishers, Philadelphia, Pa.
53.	Roizman, B., and D. Furlong. 1974. The replication of herpes viruses, p. 229-403. In H. Fraenkel-Conrat, and R. R. Wagner (ed.), Comprehensive virology. Plenum Press, New York, N.Y.
54.	Schagger, H., and G. Von Jagow. 1987. Tricine-sodium dodecyl sulfate-polyacrylamide gel electrophoresis for the separation of proteins in the range from 1 to 100 kDa. Anal. Biochem. 166:368-379[Medline].
55.	Schmolke, S., H. G. Kern, P. Drescher, G. Jahn, and B. Plachter. 1995. The dominant phosphoprotein pp65 of human cytomegalovirus. Virus Res. 69:5959-5968.
56.	Sherman, G., and S. L. Bachenheimer. 1988. Characterization of intranuclear capsids made by morphogenic mutants of HSV-1. Virology 163:471-480[Medline].
57.	Smith, J. D., and E. Harven. 1974. Herpes simplex virus and human cytomegalovirus replication in WI-38 cells. II. An ultrastructural study of viral penetration. J. Virol. 14:945-956[Abstract/Free Full Text].
58.	Sodeik, B., M. W. Ebersold, and A. Helenius. 1997. Microtubule-mediated transport of incoming herpes simplex virus 1 capsids to the nucleus. J. Cell Biol. 136:1007-1021[Abstract/Free Full Text].
59.	Spencer, J. V., W. W. Newcomb, D. R. Thomsen, F. L. Homa, and J. C. Brown. 1998. Assembly of the herpes simplex virus capsid: preformed triplexes bind to the nascent capsid. J. Virol. 72:3944-3951[Abstract/Free Full Text].
60.	Steven, A. C., C. R. Roberts, J. Hay, M. E. Bisher, T. Pun, and B. L. Trus. 1986. Hexavalent capsomers of herpes simplex virus type 2: symmetry, shape, dimensions, and oligomeric status. J. Virol. 57:578-584[Abstract/Free Full Text].
61.	Steven, A. C., J. F. Hainfeld, B. L. Trus, P. M. Steinert, and J. S. Wall. 1984. Radial distributions of density within macromolecular complexes determined from dark-field electron micrographs. Proc. Natl. Acad. Sci. USA 81:6363-6367[Abstract/Free Full Text].
62.	Steven, A. C., and P. G. Spear. 1997. Herpesvirus capsid assembly and envelopment, p. 312-351. In W. Chiu, R. M. Burnett, and R. L. Garcea (ed.), Structural biology of viruses. Oxford University Press, New York, N.Y.
63.	Tooze, J., M. Hollinshead, K. Reis, and H. Kern. 1993. Progeny vaccinia and human cytomegalovirus particles utilize early endosomal cisternae for their envelopes. Eur. J. Cell Biol. 60:163-178[Medline].
64.	Trus, B. L., F. P. Booy, W. W. Newcomb, J. C. Brown, F. L. Homa, D. R. Thomsen, and A. C. Steven. 1996. The herpes simplex virus procapsid: structure, conformational changes upon maturation, and roles of the triplex proteins VP19c and VP23 in assembly. J. Mol. Biol. 263:447-462[Medline].
65.	Trus, B. L., F. L. Homa, F. P. Booy, W. W. Newcomb, D. R. Thomsen, N. Cheng, J. C. Brown, and A. C. Steven. 1995. Herpes simplex virus capsids assembled in insect cells infected with recombinant baculoviruses: structural authenticity and localization of VP26. J. Virol. 69:7362-7366[Abstract].
66.	Vernon, S. K., W. C. Lawrence, C. A. Long, B. A. Rubin, and J. B. Sheffield. 1982. Morphological components of herpesvirus. IV. Ultrastructural features of the envelope and tegument. J. Ultrastruct. Res. 81:163-171[Medline].
67.	Weiner, D., and W. Gibson. 1983. Phosphorylation, maturational processing, and relatedness of strain Colburn matrix proteins. Virology 129:155-169[Medline].
68.	Welch, A. R., L. M. McNally, and W. Gibson. 1991. Cytomegalovirus assembly protein nested gene family: four 3'-coterminal transcripts encode four in-frame, overlapping proteins. J. Virol. 65:4091-4100[Abstract/Free Full Text].
69.	Welch, A. R., A. S. Woods, L. M. McNally, R. J. Cotter, and W. Gibson. 1995. A herpesvirus maturational protease, assemblin: identification of its gene, putative active site domain, and cleavage site. Proc. Natl. Acad. Sci. USA 88:10792-10796[Abstract/Free Full Text].
70.	Wingfield, P. T., S. J. Stahl, D. R. Thomsen, F. L. Homa, F. P. Booy, B. L. Trus, and A. C. Steven. 1997. Hexon-only binding of VP26 reflects differences between the hexon and penton conformations of VP5, the major capsid protein of herpes simplex virus. J. Virol. 71:8955-8961[Abstract].
71.	Wood, L. J., M. K. Baxter, S. M. Plafker, and W. Gibson. 1997. Human cytomegalovirus capsid assembly protein precursor (pUL80.5) interacts with itself and with the major capsid protein (pUL86) through two different domains. J. Virol. 71:179-190[Abstract].
72.	Zhou, Z. H., B. V. V. Prasad, J. Jakana, F. J. Rixon, and W. Chiu. 1994. Protein subunit structures in the herpes simplex virus capsid determined from 400-kV spot-scan electron cryomicroscopy. J. Mol. Biol. 242:456-469[Medline].
73.	Zhou, Z. H., J. He, J. Jakana, J. D. Tatman, F. J. Rixon, and W. Chiu. 1995. Assembly of VP26 in herpes simplex virus-1 inferred from structures of wild-type and recombinant capsids. Nat. Struct. Biol. 2:1026-1030[Medline].