Role of Pseudorabies Virus Us9, a Type II Membrane Protein, in Infection of Tissue Culture Cells and the Rat Nervous System

doi:10.1128/JVI.74.2.834-845.2000

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Journal of Virology, January 2000, p. 834-845, Vol. 74, No. 2
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Role of Pseudorabies Virus Us9, a Type II Membrane Protein, in Infection of Tissue Culture Cells and the Rat Nervous System

A. D. Brideau,¹ J. P. Card,² and L. W. Enquist¹^,^*

Department of Molecular Biology, Princeton University, Princeton, New Jersey 08544,¹ and Departments of Neuroscience and Psychiatry, University of Pittsburgh, Pittsburgh, Pennsylvania 15260²

Received 19 July 1999/Accepted 25 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The protein product of the pseudorabies virus (PRV) Us9 gene is a phosphorylated, type II membrane protein that is insertedinto virion envelopes and accumulates in the trans-Golgi network.It is among a linked group of three envelope protein genes inthe unique short region of the PRV genome which are absent fromthe attenuated Bartha strain. We found that two different Us9null mutants exhibited no obvious phenotype after infection ofPK15 cells in culture. Unlike those of gE and gI null mutants,the plaque size of Us9 null mutants on Madin-Darby bovine kidneycells was indistinguishable from that of wild-type virus. However,both of the Us9 null mutants exhibited a defect in anterogradespread in the visual and cortical circuitry of the rat. The visualsystem defect was characterized by restricted infection of a functionallydistinct subset of visual projections involved in the temporalorganization of behavior, whereas decreased anterograde spreadof virus to the cortical projection targets was characteristicof animals receiving direct injections of virus into the cortex.Spread of virus through retrograde pathways in the brain was notcompromised by a Us9 deletion. The virulence of the Us9 null mutants,as measured by time to death and appearance of symptoms of infection,also was reduced after their injection into the eye, but not aftercortical injection. Through sequence analysis, construction ofrevertants, measurement of gE and gI protein synthesis in theUs9 null mutants, and mixed-infection studies of rats, we concludethat the restricted-spread phenotype after infection of the ratnervous system reflects the loss of Us9 and is not an indirecteffect of the Us9 mutations on expression of glycoproteins gEand gI. Therefore, at least three viral envelope proteins, Us9,gE, and gI, function together to promote efficient anterogradetransneuronal infection by PRV in the rat central nervoussystem.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Pseudorabies virus (PRV) is a neurotropic alphaherpesvirus of the Herpesviridae family that is able to infect neurons of boththe peripheral and central nervous systems of a wide variety ofmammals and birds (4, 39). When PRV replicates and spreadsin the nervous system, it acts as a self-amplifying tracer ofsynaptically connected neurons (10, 16). Integral to thisprocess is the demonstrated ability of the virus to exploit thepolarized cellular architecture of neurons and move throughoutthe brain of a host organism. Thus, assays of the spread of virusthrough the brain naturally incorporate a determination of thedirection of viral transport through a circuit. Direction in thenervous system is defined by the terms "anterograde" and "retrograde,"which can be used to describe directional movement of virus insidea cell as well as the spread of virus between synaptically connectedneurons. We use the terms anterograde spread and retrograde spreadin this report to describe movement of virus between synapticallyconnected neurons. Spread from the primary infected neuron tothe second-order uninfected neuron in the direction of the nerveimpulse is taken to be anterograde spread. Spread in the oppositedirection, against the direction of the nerve impulse, is describedas retrograde spread. In this report, both of these terms areused to describe the direction of transynaptic viral transportthrough two model circuits that we have developed to study therole of PRV-encoded envelope proteins in directional spread ofvirus in the rat nervoussystem.

Hints that viral gene products affect the direction of spread in herpesvirus neuronal infections come from several studies.For instance, differential-spread patterns for two strains ofherpes simplex virus type 1 (HSV-1) have been noted both in theprimate motor system and in the murine optic pathway (17, 46).However, neither of these phenotypes has yet been associated withspecific HSV-1 gene products. Studies in our laboratory have demonstratedthat an attenuated PRV strain called PRV Bartha selectively infectsa restricted subset of neurons in the rat visual system (12)and the rat prefrontal cortex (PFC) (9). Similarly, Rotto-Percelayand colleagues (40) demonstrated a restricted invasion by PRVBartha of neurons innervating the gastrocnemius muscle of rats.In that analysis, virus replicated efficiently in motor and autonomicneurons innervating the muscle but did not replicate in neuronsin the dorsal root ganglia (DRG) that provide the sensory innervationof the muscle. Importantly, PCR analysis in that study demonstratedPRV DNA in the sensory neurons. We have further demonstrated thatwild-type virus (PRV Becker), but not PRV Bartha, injected intoneck musculature of a cat replicates efficiently in DRG neuronsserving the inoculated muscles (8). Several laboratories havedemonstrated that the absence of the gE and gI genes from PRVBartha accounts for the restricted spread in neurons in a varietyof animal models (1, 3, 10, 12, 22, 25, 26, 29,31, 45).

The PRV Bartha strain carries a large deletion in the unique short region of the genome that removes not only the gE and gIcoding sequences but also all of the Us9 gene and part of theUs2 coding sequences (27, 29, 34). While the phenotypesof individual null mutants of gE, gI, and Us2 have been analyzed,the phenotype of a PRV Us9 null virus in an otherwise wild-typebackground has never been reported. All previously characterizedUs9 mutant viruses contained additional mutations, especiallyin the neighboring genes, the gI and gE genes (30, 32, 35-37,43). Therefore, to determine the Us9 null phenotype in vitroand in vivo, we constructed two isogenic strains of PRV Beckercontaining defined mutations in the Us9 gene. PRV 160 containsa nonsense mutation at amino acid 4, and PRV 161 contains a deletionremoving the majority of the Us9 gene open reading frame. In thisreport, we used these two mutants and their revertants to determineif the Us9 protein plays any role in infection of standard tissueculture cell lines and in directional transneuronal infectionof the rodent nervous system by using two well-characterized modelsof PRV invasiveness. We demonstrate that while mutants lackingthe PRV Us9 gene have no obvious phenotypes in tissue culturecells, the mutants are defective in anterograde spread in visualand corticalcircuitry.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Virus strains and cells. Pig kidney (PK15) cells and Madin-Darby bovine kidney (MDBK) cells were grown in Dulbecco's modified Eagle medium (DMEM) supplementedwith 10% fetal bovine serum (FBS). All viruses used in this studywere propagated on PK15 cells in DMEM containing 2% FBS as previouslydescribed (45). PRV 91 contains a deletion removing the gE geneopen reading frame and has been described previously (11). PRV98 contains a deletion removing the gI gene open reading frame(45).

Antisera. The rabbit polyvalent and mouse monoclonal Us9 antisera have been described previously (5, 6). The gE monoclonal pool(M133, M138, M156) was received from T. Ben-Porat. The rabbitpolyvalent gE and gI antisera were kindly provided by K. Bienkowska-Szewczyk(University of Gdansk). Rb133 is a rabbit polyvalent antiserumagainst acetone-inactivated PRV Becker and recognizes all of themajor envelope glycoproteins (11). The polyvalent goat PRV gB(Ab 284) antiserum has been described previously (38).

Virus construction and characterization. (i) Construction of PRV 160 and PRV 161. PRV 160 is an isogenic strain of PRV Becker which does not express the Us9 protein due to insertion of a nonsense codon atamino acid 4 in the Us9 open reading frame (Fig. 1). To constructPRV 160, a transfer vector in which the phenylalanine (TTC) codonat position 4 of the Us9 open reading frame was changed to a nonsensestop codon (TAA) by site-directed mutagenesis was first engineered.Specifically, oligonucleotide mutagenesis was performed with theAltered Sites kit (Promega) on plasmid pRS3 containing the SphI-MluIregion of the PRV BamHI 7 fragment (41). The oligonucleotide(Us9 AflII-1) used to introduce the nonsense stop codon at position4 also introduced a unique AflII restriction enzyme site at position3 of the Us9 open reading frame. Addition of the AflII site facilitatedthe screening of mutated clones and the confirmation of recombinantviruses. The mutagenized pRS3 plasmid was digested with restrictionenzymes SphI and MluI to release a 1,004-bp fragment containingthe Us9 gene with the nonsense stop codon at position 4. Thisfragment was then used to replace the SphI-MluI fragment of pPH2,and the resulting plasmid was named pAB24. pPH2 contains the SalI-MluIregion of the PRV Becker BamHI 7 fragment encompassing a portionof the gD gene; the gI, gE, and Us9 genes; and the 5' end of theUs2 gene. The nucleotide sequence of the mutagenized SphI-MluIfragment was confirmed by DNA sequencing with Sequenase (UnitedStates Biochemical). The pAB24 transfer vector was cotransfectedby the calcium phosphate method (18) with PRV 91 viral DNA,in which the gE sequences are deleted, and the infected cellsand medium were collected when total cytopathic effect was observed.The virus stock was replated onto PK15 cells, and recombinantviruses were screened for gE expression by an immunoreactivityassay with a gE monoclonal pool. gE immunoreactive plaques werepicked and plaque purified five times.

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FIG. 1. PRV genome and map of virus strains used in this study. The BamHI 7 fragment of the unique short (US) region is expanded to show the genes contained in this fragment. The US deletion of PRV Bartha (Ba) is indicated by a black box. PRV 91 contains a deletion removing the gE coding sequences. PRV 98 is a gI null virus. PRV 160 contains a nonsense stop mutation (stop) at position 4 in place of a phenylalanine residue (F) in the Us9 open reading frame. PRV 161 contains a 258-bp deletion in the Us9 open reading frame. Relevant restriction enzyme sites used in construction of the various recombinant viruses are indicated. UL, unique long region; PRV Be, PRV Becker; IR, internal repeat.

PRV 161 is an isogenic strain of PRV Becker which does not express the Us9 protein due to a 258-bp deletion (from a totalof 294 bp in the Us9 gene open reading frame) removing the nucleotidesequence encoding amino acids 4 through 89 of the Us9 gene openreading frame (Fig. 1). To construct PRV 161, a transfer vectorwas constructed by site-directed mutagenesis on plasmid pRS3 asdescribed above for the construction of PRV 160. As for PRV 160,oligonucleotide Us9 AflII-1 was used to introduce an AflII restrictionsite at position 3 followed by a nonsense codon at position 4in the Us9 gene open reading frame. In addition, a second oligonucleotide(Us9 AflII-2) was used in the same mutagenesis reaction to introducean additional AflII site near the 3' end of the Us9 gene at position89. The resulting mutagenized plasmid, therefore, contained anAflII restriction site at both the 5' and 3' ends of the Us9 gene.Digestion of the doubly mutagenized plasmid with AflII releaseda 258-bp fragment containing the majority of the Us9 gene. TheAflII-digested plasmid was then self-ligated, resulting in a plasmidwith base pairs 8 through 267 of the Us9 gene deleted. The SphI-MluIfragment of this plasmid was then used to replace the correspondingfragment of pPH2, thereby constructing the final transfer vector,pAB25. Plasmid AB25 was cotransfected with PRV 91 viral DNA, andgE-immunoreactive plaques were picked and plaque purified as describedabove for PRV160.

(ii) Construction of PRV 160 and PRV 161 revertants. PRV 160R and PRV 161R are isogenic strains of PRV 160 and PRV 161, respectively, in which the mutated Us9 gene was replacedwith wild-type Us9 gene sequences by homologous recombination.PRV 160R and PRV 161R were created by cotransfection of eitherPRV 160 or PRV 161 viral DNA and a gel-purified SphI-MluI PRVBecker fragment. The 1,004-bp SphI-MluI fragment spans from thegE gene cytoplasmic tail to the beginning of the Us2 gene. Recombinantviruses were screened for with a black-plaque immunoreactivityassay with polyvalent Us9 antiserum. Both PRV 160R and PRV 161Rwere subjected to five rounds of plaquepurification.

(iii) Southern blot analysis. Southern blot analysis was used to confirm the desired mutations in all the viruses described above. Both the nonsense mutationin PRV 160 and the deletion in PRV 161 created a novel AflII sitein the Us9 gene. For PRV 160, digestion of the BamHI 7 fragmentwith AflII converts a 6,613-bp fragment to two fragments of 5,708and 905 bp. For PRV 161, the 6,355-bp BamHI 7 fragment is cleavedby AflII into a 5,708-bp fragment and a 647-bp fragment. PRV 160Rand PRV 161R were examined by Southern blot analysis for the lossof the unique AflII site in the BamHI 7fragment.

(iv) Black-plaque immunoreactivity assay. Monolayers of PK15 cells were infected with virus to yield approximately 500 plaques per 10-cm-diameter dish and were overlayedwith DMEM containing 1% Methocel and 2% FBS. After approximately48 h, the Methocel solution was aspirated and the plaques werewashed three times with phosphate-buffered saline (PBS). The plaqueswere then incubated in primary antibody for 1 h at room temperatureon a rocking platform. For gE immunoreactivity assays, the gEmonoclonal pool was first mixed 1:1:1 and then diluted 1:10 inPBS containing 3% bovine serum albumin (BSA). For Us9 immunoreactivityassays, the rabbit polyvalent Us9 antiserum was diluted 1:200in PBS plus 3% BSA. After incubation with the primary antibody,the plaques were washed three times with PBS and incubated ina peroxidase-labeled goat anti-mouse (gE monoclonal pool) or anti-rabbit(Us9) secondary antibody (Kirkegaard and Perry) diluted 1:200in PBS plus 3% BSA. Following a 1-h incubation in the secondaryantibody, the plates were rinsed three times with PBS and theimmunoreactive plaques were detected by the addition of a detectionsolution containing 10 mg of 4-chloro-1-naphthol (Sigma)/ml and0.3% hydrogen peroxide. Positive plaques were picked and resuspendedin 1 ml of DMEM plus 2%FBS.

(v) Plaque size determination. Monolayers of MDBK cells in 60-mm-diameter dishes were infected with virus to yield approximately 200 plaques per dish. Afterapproximately 48 h of infection, the plaques were visualized bya black-plaque immunoreactivity assay with gB antiserum (1:200).The assay was performed essentially as described above exceptthat the plaques were first treated with 2% paraformaldehyde for10 min at room temperature to fix the cells prior to additionof the primary antibody (diluted in PBS containing 3% BSA and0.5% saponin). The diameters of 20 random immunoreactive plaqueswere measured on an Olympus inverted microscope with an ocularreticule.

(vi) Western blot analysis. Monolayers of PK15 cells were infected with PRV Becker, PRV 160, PRV 161, PRV 160R, or PRV 161R at a multiplicity of infection(MOI) of 10. At 15 h after infection, the cells were washed withPBS and harvested in lysis buffer (150 mM NaCl, 10 mM Tris [pH7.8], 1% Triton X-100, 1% sodium deoxycholate). Viral particleswere isolated from the medium of infected cells by centrifugationthrough sucrose as described previously (5). Approximately10 µg of total cellular extract or 1 µg of purified virions wasseparated on a sodium dodecyl sulfate (SDS)-12.5% polyacrylamidegel and transferred to nitrocellulose (Amersham) by a semidrytransfer apparatus. The Us9, gE, and gI proteins were visualizedby incubation of the nitrocellulose with primary antibodies followedby enhanced chemiluminescence detection (SuperSignal;Pierce).

Animal infections. (i) Animals. Adult male Sprague-Dawley rats weighing 210 to 290 g were used in this assay. The photoperiod was standardized to 14 h oflight and 10 h of dark (light on at 0600 h). Food and water werefreely available throughout the experiments. Experimental protocolswere approved by the Animal Welfare Committees at Princeton Universityand the University of Pittsburgh and were consistent with theregulations of the American Association for Accreditation of LaboratoryAnimal Care and those in the Animal Welfare Act (Public Law 99-198).During the course of the experiment, all animals were confinedto a biosafety level 2 laboratory and experiments were conductedwith the specific safeguards noted by Enquist and Card (14).Animals were deeply anesthetized by intraperitoneal or intramuscularinjection of ketamine (60 mg per kg of body weight) and xylazine(7 mg/kg) prior to all experimentalmanipulations.

(ii) Intravitreal injections. Injection of PRV Becker into the vitreous humor of the rat eye leads to first-order infection of retinal ganglion cells andsubsequent anterograde transynaptic infection of all regions ofthe brain that receive retinal input (10, 12). Infection ofretinorecipient nuclei occurs in two separated waves that targetthe dorsal geniculate nucleus (DGN) and superior colliculus (SC),areas involved in visual perception and reflex movements of theeyes, followed by regions of the diencephalon (suprachiasmaticnuclei [SCN] and intergeniculate leaflets [IGL]) responsible forimparting temporal organization to behavior and physiologicalprocesses (10, 12). Identical injection of PRV Bartha andstrains isogenic with PRV Becker but lacking gE or gI producesa restricted pattern of central infection characterized by replicationof virus in the SCN and the IGL and a failure of virus to replicatein the DGN or SC (10-12, 45). Using this model, we examined theinvasiveness of the Us9 mutants in 11 rats. Infection of the retinawas performed as described previously (12). Briefly, 2.5 µlof virus (approximately 10⁸ to 10⁹ PFU/ml) was injected into the vitreous humor of the left eyesof anesthetized animals with a Hamilton microliter syringe equippedwith a 26-gauge sharpened needle. The inoculum was injected slowlyover a period of 10 min, and the needle was left in the eye foran additional 10 min in an effort to reduce leakage of virus intothe orbit. Four additional animals received intravitreal injectionof 4 µl of either PRV 160 or PRV 161 (two animals each) to determineif the viral concentration affected the pattern of anterogradeinfection. For the complementation experiments, a 1:1 (vol/vol)mixture of PRV 161 (4 × 10⁸ PFU/ml) and either PRV 91 (gE null; 6 × 10⁸ PFU/ml) or PRV 98 (gI null; 7 × 10⁸ PFU/ml) was prepared just prior to inoculation. The animals wereanesthetized and killed by transcardiac infusion of buffered aldehydesolutions when symptoms of infection were overt. Survival timesfor animals infected with wild-type virus or with Us9 null strainsranged from 60 to 86 h and 67 to 112 h, respectively. The brainswere then removed and prepared for immunohistochemical localizationof infected neurons by procedures detailedbelow.

(iii) PFC injections. Anterograde transneuronal spread of viral mutants resulting from intracerebral injection of mutants into the PFC was characterizedin 35 rats. This model takes advantage of the unidirectional projectionbetween the PFC and the subjacent striatum and was used in a prioranalysis to demonstrate differences in the levels of invasivenessof PRV Bartha and PRV Becker (9). The basic organization ofthe circuitry that it is based upon is described in that paper.Injections were conducted in the following manner according tothe methods established by Card and colleagues (9). The headsof anesthetized animals were secured in a stereotaxic frame, and100 to 200 nl of virus was injected into the medial PFC by usingcoordinates derived from the rat brain atlas of Paxinos and Watson(33). Virus was injected slowly over a period of 5 min witha 1-µl syringe equipped with a 26-gauge sharpened needle, andthe needle was left in the brain for 10 min following completionof the injection to reduce reflux of the inoculum along the injectiontract. After survival times of 47 to 66 h, animals were anesthetizedand killed for immunohistochemical localization of infected neuronsby the procedures describedbelow.

(iv) Immunohistochemical procedures. Following transcardiac perfusion fixation with buffered paraformaldehyde solutions the brain was postfixed in the primaryfixative and cryoprotected in a 20% phosphate-buffered sucrosesolution. Each brain was then sectioned serially in the coronalplane with a freezing microtome at 35 µm. Six bins of tissue werecollected and transferred to a glycol-based cryopreservant (44)and stored at $-$ 20°C until they were processed for immunohistochemicallocalization of infected neurons. We have previously shown thatthis method of tissue storage preserves the antigenicity of viralantigens for a minimum of 6 years. One bin of sections (a sectionfrequency of 210 µm) was processed for immunohistochemical localizationof infected neurons with a rabbit polyclonal antiserum (Rb133)generated against acetone-inactivated PRV Becker. This procedureutilized the avidin-biotin immunoperoxidase procedure developedby Hsu and colleagues (19), species-specific affinity-purifiedsecondary antibodies (Jackson ImmunoResearch), and VectastainElite reagents (Vector Laboratories). After immunoperoxidase processing,sections were mounted on gelatin-coated slides, dehydrated witha graded ethanol series, cleared with xylene, and coverslippedwith Cytoseal60 (Stephens Laboratories). Specific details regardingthis procedure have been published previously (7, 14).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of Us9 null viruses. We constructed isogenic strains of PRV Becker containing two different null mutations in the Us9 gene. As the transcriptionof this region is complex and not well understood, deletion mutationsmay alter local transcripts qualitatively and quantitatively.Accordingly, we constructed a Us9 nonsense mutant as well as adeletion mutant to increase confidence that the phenotypes wedetermined reflected the loss of Us9 expression. PRV 160 containsa nonsense mutation at position 4 of the Us9 open reading frame.PRV 161 contains a 258-bp deletion removing the majority of theUs9 coding sequences. The construction of these viruses is describedin Materials and Methods (Fig. 1).

Us9 null viruses express gE and gI proteins. To ensure that PRV 160 and PRV 161 no longer expressed the Us9 protein yet maintained wild-type expression levels of the gEand gI proteins, we examined the steady-state levels of Us9, gE,and gI in PRV Becker-, PRV 160-, and PRV 161-infected cells. Celllysates were prepared from monolayers of PK15 cells infected withPRV Becker, PRV 160, or PRV 161 at an MOI of 10 and were Westernblotted with Us9, gE, or gI antiserum. As anticipated, Us9-immunoreactivepolypeptides were detected in PRV Becker-infected PK15 cells butwere absent from PRV 160- and PRV 161-infected cell lysates (Fig.2A). The Us9 protein is present in PRV Becker-infected cell lysatesas three polypeptides ranging from approximately 17 to 20 kDa.Western blot analysis with gE and gI antisera revealed that PRVBecker, PRV 160, and PRV 161 all produced identical species ofboth the gE and gI proteins (Fig. 2A). The gE protein is presentin infected cell lysates as both an immature precursor from migratingat approximately 93 kDa and a mature glycosylated form migratingat approximately 110 kDa. The gI protein is expressed as a 65-kDaprecursor that is glycosylated to a mature form, which is notwell recognized by the gI antiserum used in this experiment. Asthe steady-state levels of the gE and gI proteins in the PRV 160-and 161-infected cells are indistinguishable from those in PRVBecker-infected cells, we are confident that the engineered mutationsin the Us9 gene did not interfere with expression of either gEor gI proteins. The expression and processing of the glycoproteinsgB and gC were also unaffected by the loss of Us9 (data not shown).Figure 2B shows the result of Western blot analysis with Us9-specificantiserum of PK15 cells infected with PRV Becker, PRV 160, PRV161, and the revertant viruses PRV 160R and PRV 161R. The wild-typesteady-state level of the Us9 protein in both PRV 160R and PRV161R clearly demonstrates that the full-length Us9 gene has beenrestored to these viruses.

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FIG. 2. Western blot analysis of Us9 null viruses and revertants. Monolayers of PK15 cells were infected with PRV Becker, PRV 160, and PRV 161 (A and B) and the revertant viruses PRV 160R and PRV 161R (B) at an MOI of 10. Cellular extracts were prepared after 15 h of infection, and approximately 10 µg of total cell lysate was fractionated on an SDS-12.5% polyacrylamide gel, transferred to nitrocellulose, and analyzed by Western blotting with gE, gI, or Us9 antiserum. (C) Viral particles were isolated from the medium of PK15 cells infected for 15 h with either PRV Becker, PRV 160, or PRV 161 (MOI = 10) by centrifugation through sucrose. Virions were analyzed by Western blotting with either gE or Us9 antiserum. The migration of molecular mass markers is indicated on the left in kilodaltons.

We also examined purified viral particles by Western blot analysis to ensure that the absence of the Us9 protein did not interferewith the incorporation of other glycoproteins into the virionenvelope. Specifically, we isolated virions from the medium ofPK15 cells infected with PRV Becker, PRV 160 and PRV 161 (MOI= 10) by centrifugation through sucrose. The purified virionswere separated on an SDS-12.5% polyacrylamide gel and Westernblotted with antisera against Us9 and gE. As anticipated, onlyPRV Becker virions incorporated Us9 into the viral envelope asPRV 160 and PRV 161 do not express the Us9 protein (Fig. 2C).Western blot analysis with gE-specific antiserum revealed thatgE was efficiently incorporated into both PRV 160 and PRV 161viral particles despite the absence of Us9 (Fig. 2C). Furtherexamination of these viral particles showed that the absence ofUs9 also did not affect the incorporation of either the gI orgC membrane proteins into the virion envelope (data notshown).

Us9 null mutants have no observable defects in growth or cell-to-cell spread. The ability of a virus to form plaques on monolayers of cultured epithelial cells is believed to reflect cell-to-cell spreadof a virus in vivo. PRV gE and gI null viruses replicate as wellas wild-type virus in single-step growth experiments but formsmall plaques on MDBK cells (20, 21, 47). We performed single-stepgrowth analysis with PRV 160 on PK15 cells. PRV 160 produced andreleased equivalent amounts of virus with the same kinetics asthose observed for both the wild-type strain, PRV Becker, andthe revertant strain PRV 160R (data not shown). To test if theUs9 null viruses have a defect in cell-to-cell spread as measuredby plaque size in tissue culture, confluent monolayers of MDBKcells were infected with approximately 200 PFU of PRV Becker,PRV 160, or PRV 161. The sizes of PRV Bartha and PRV 91 plaqueson MDBK cells were also measured for comparison. The results ofthis experiment are shown in Table 1. Unlike PRV Bartha and PRV91, which form significantly smaller plaques on MDBK cells thanPRV Becker (36 and 74% of wild type, respectively), both PRV 160and PRV 161 formed plaques that were indistinguishable from thoseof PRV Becker in both shape and size.

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TABLE 1. Plaque size on MDBK cells

Anterograde transneuronal spread of PRV 160 and PRV 161 through visual projections. To determine if the Us9 protein plays a role in anterograde spread in the visual system, we injected the Us9 null viruses,PRV 160 and PRV 161, into the vitreous humor and examined theresulting pattern of infection in the brain as described in Materialsand Methods. Specifically, we injected 2.5 × 10⁵ to 10⁶ PFU of PRV 160 or PRV 161 (Table 2) into the vitreous body andcharacterized the central patterns of infection at survival timesextending from 67 to 112 h postinoculation. PRV Becker (1.2 ×10⁶ PFU) and PRV 91 (5 × 10⁵ PFU) were injected into separate groups of animals as controls(Table 2). At the time of imminent death, the animals were sacrificedand the brains were removed, fixed, and prepared for immunohistochemicallocalization of infected neurons. PRV Becker and PRV 91 producedthe expected patterns of central infection. Viral antigen wasdetected in all retinorecipient areas in PRV Becker-infected animals,whereas virus was restricted to the SCN and IGL of animals infectedwith PRV 91 (Fig. 3). PRV 160 and PRV 161 produced a restrictedpattern of infection essentially identical to that produced byPRV 91 and other mutants lacking gE or gI (10-12, 45). Both ofthe Us9 null mutants produced a robust infection of the SCN andIGL but failed to produce productive replication of virus in theDGN and SC, even though the postinoculation survival intervalssubstantially exceeded those shown to be adequate for infectionof these areas with PRV Becker. Injection of a larger amount ofvirus (2 × 10⁶ to 5 × 10⁶ PFU in 4 µl) produced the same restricted phenotype, demonstratingthat the failure to infect neurons in the DGN and SC was not relatedto the concentration of the inoculum.

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TABLE 2. Intravitreal injections

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FIG. 3. Anterograde transport of Us9 null viruses in the rodent visual system. Approximately 2.5 × 10⁵ to 2 × 10⁶ PFU of PRV Becker (Be), PRV 91, PRV 160, or PRV 161 was injected into the vitreous humor of Sprague-Dawley male rats. At the time of imminent death, the animals were sacrificed, and the brains were fixed and sliced into 35-µm-thick coronal sections with a freezing microtome. Viral antigen was detected with rabbit polyvalent antiserum Rb133. Representative sections are shown for each virus. LGN, lateral geniculate nuclei; D, dorsal; V, ventral.

The restricted-spread phenotype reflects absence of Us9. Several measures were taken to ensure that the phenotype observed for the Us9 null viruses was due to the absence of Us9 ratherthan other mutations. We were particularly concerned that unexpectedmutations may have been introduced into the adjacent gE gene duringconstruction of the viruses. First, we sequenced the plasmidscontaining the Us9 mutations that were used for construction ofthe recombinant viruses in their entirety in both directions.This analysis demonstrated that there were no additional mutationsin regions adjacent to the Us9 mutations in PRV 160 and PRV 161.Second, we constructed revertants of both Us9 mutants by reintroducingthe wild-type Us9 gene by homologous recombination. To constructthe revertants, PRV 160 or PRV 161 viral DNA was cotransfectedwith a 1,004-bp fragment of PRV Becker DNA containing the completeUs9 gene sequence as well as 373 bp of upstream flanking gE geneand intergenic sequences and 334 bp of downstream flanking intergenicand Us2 gene sequences. Revertants PRV 160R (data not shown) andPRV 161R (Fig. 4) both produced the wild-type pattern of braininfection after injection into the vitreous body.

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FIG. 4. Reversion and complementation analysis of the Us9 null spread defect. The spread patterns of virus following intraocular injection of animals with PRV Becker (Be), PRV 161, PRV 161R, and a 1:1 (vol/vol) mixed population of PRV 161 and PRV 91 are shown. The infected tissue was processed and analyzed as described in the legend for Fig. 3. Abbreviations are as used for Fig. 3.

Pair-wise, mixed infection of individual mutants restores wild-type spread. To further test that the spread defect observed for the two Us9 null mutants was due to the absence of Us9 and not becausethe mutations affected the adjacent gE and gI genes, we used mixed-infectionexperiments with pairs of gE, gI, and Us9 null mutants as describedby Enquist et al. (15). The mixed-infection experiments alsotested the hypothesis that the restricted spread of PRV 160 andPRV 161 is due to the lack of Us9 in their viral envelopes suchthat they no longer can enter into the retinal ganglion cellsthat project to the DGN and the SC. As demonstrated in Fig. 3,viruses, examined individually in the rat visual system, thatlack either gE (PRV 91) or Us9 (PRV 160 and PRV 161) are incapableof infecting the DGN or SC. In the experiment shown in Fig. 4,a 1:1 mixture of a Us9 null virus (PRV 161) and a gE null virus(PRV 91) was injected into the vitreous body. When the animalswere exhibiting terminal symptoms, they were euthanized, and theirbrains were examined for extent of virus spread. We observed markedrestoration of anterograde spread of infection to both the DGNand the SC in animals that were injected with both mutant viruses.The smaller numbers of PRV-positive neurons in the DGN and SCof animals coinfected with PRV 91 and PRV 161 compared to thoseof animals infected with the wild-type strain, PRV Becker, mostlikely reflects the inefficiency of complementation and the architectureof the circuitry. Whereas both the SC and DGN are infected byanterograde transneuronal passage of virus through retinal ganglioncells, the DGN also receives projections from the SC. Therefore,infection of animals with the wild type strain, PRV Becker, canproduce a direct anterograde infection of the DGN through retinalganglion cells and an indirect infection through the SC. However,in a complementation experiment, both Us9 null and gE null virusesneed to enter the same retinal ganglion cell to produce complementedvirus that can spread in the anterograde direction to the SC andDGN, and the same process has to occur for indirect infectionof the DGN through the SC. We also performed a similar mixed infectionwith PRV 161 (Us9 null) and PRV 98 (gI null) and observed fullrestoration of spread to all retinorecipient regions (data notshown). Taken together, these experiments strongly suggest thatUs9 is not needed to enter retinal ganglion cells projecting tothe visual centers and therefore that the anterograde spread defectassociated with the loss of Us9 must occur after viral entry.Moreover, these results further confirm that the gE and gI genesin the Us9 null viruses are fully functional and that the restrictedanterograde spread observed for PRV 160 and PRV 161 is due tothe loss of the Us9protein.

Directional spread of Us9 mutants injected into the PFC. Injection of Us9 null mutants into the PFC permitted an assessment of the role of this envelope protein in both anterogradeand retrograde transport through cortical circuits. As demonstratedpreviously, anterograde transynaptic passage of virus can be determinedby the extent of infection in the striatum, an area that receivesa projection from the prefrontal cortex but that does not reciprocatethe projection (9). Retrograde transynaptic passage of thisvirus through projections to the PFC from other regions of thecortex and the thalamus were also accurately measured. Two daysfollowing injection of 100 or 200 nl of PRV Becker into the PFC,infected neurons were observed in the striatum in a pattern overlappingthe known distribution of axons that project to this region fromthe PFC. Importantly, the magnitude of infection was concentrationdependent, with a larger number of infected neurons present inanimals infected with 200 nl of PRV Becker (Fig. 5). Deletionof either Us9 or gE reduced the magnitude of anterograde transneuronalinfection of striatal neurons and also delayed the temporal sequenceof infection (Fig. 6). A similar reduction in anterograde spreadto striatal neurons was also observed for a gI null virus (PRV98) (data not shown). In all cases, the striatum was free of infectedneurons at 24 h and contained only a moderate number of infectedstriatal neurons in the longest-surviving animals. For example,66 h after injection of PRV 91, there were only scattered infectedstriatal neurons, which were confined to the region that receivesa projection from the injected region of PFC. A similar reductionin anterograde infection of this area was noted 50 and 55 h afterinjection of 100 nl of PRV 161 and PRV 160 (Fig. 6C and D andE and F, respectively). Examination of longer postinoculationintervals with these viruses was not possible given the increasedvirulence of PRV 160 and PRV 161 compared to that of PRV 91 orPRV 98 (see below). Importantly, injecting larger concentrationsof the Us9 null mutants did not increase the magnitude of anterogradetransynaptic infection of the striatum as it did with PRV Becker.This is readily apparent by comparing the restricted pattern ofstriatal infection 49 h after the injection of 200 nl of PRV 160(Fig. 6G and H) with the extensive anterograde striatal infection47 h after injection of an equivalent amount of PRV Becker (Fig.5A and B).

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FIG. 5. The extent of anterograde transneuronal infection of the striatum approximately 48 h after injection of 100 (C and D) or 200 nl (A and B) of PRV Becker into the PFC. The areas of the striatum indicated by the arrows in panels A and C are shown at higher magnification in panels B and D, respectively. Note that the extent of anterograde transneuronal infection of the striatum was dramatically increased by injection of the higher concentration of virus. Bars: A and C, 550 µm; B and D, 20 µm.

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FIG. 6. The extent of anterograde transneuronal infection of striatal neurons following injection of PRV 91 (A and B), PRV 161 (C and D), or PRV 160 (E and F) into the medial PFC. The areas of the striatum indicated by the arrows in panels A, C, E, and G are shown at higher magnification in panels B, D, F, and H, respectively. Note that the relative magnitudes of striatal infection produced by injection of 100 nl of PRV 160 or PRV 161 into PFC are similar at 50 to 55 h following injection (compare panels C and D with E and F). In contrast, 66 h was required to achieve a similar magnitude of anterograde infection after injection of PRV 91. It is also important to note that injection of 100 (E and F) or 200 nl (G and H) of PRV 160 into the PFC produced similar magnitudes of anterograde transneuronal infection in the striatum. This contrasted with the concentration-dependent differences in the extent of infection produced by PRV Becker (Fig. 5). Bar in A, 500 µm (same scale for panels C, E, and G); bar in B, 20 µm (same scale for panels D, F, and H).

Although deletion of Us9, gE, or gI produced a comparable disruption in anterograde transynaptic infection of striatal neurons,the effects of these deletions upon retrograde spread of virusdiffered. Rats injected with PRV 91 exhibited delayed retrogradetransynaptic transport of virus relative to animals infected withPRV Becker. Whereas PRV Becker exhibited extensive retrogradespread of virus by 48 h (data not shown, but see reference 9),the gE null mutant produced a much more restricted infection ofthe same circuitry at this postinoculation interval and only achieveda magnitude of retrograde infection equivalent to that of wild-typevirus at 66 h (Fig. 7A to C). Similarly, 66 h was required forPRV 91 to produce a retrograde spread of virus that was equivalentto that produced by PRV 160 or PRV 161 at 55 and 50 h, respectively(Fig. 7D to F and G to I).

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FIG. 7. Extent of retrograde infection of thalamus and perirhinal cortex following injection of PRV 91 (A to C), PRV 160 (D to F), or PRV 161 (G to I) into PFC. The boxed areas shown in panel A designate the regions of the thalamus and perirhinal cortex shown at higher magnification in the photomicrographs to the right in each row (thalamus in panels B, E, and H; perirhinal cortex in panels C, F, and I). Note that the levels of retrograde infection produced by all three viruses are similar even though the animal infected with PRV 91 survived 66 h and those injected with PRV 160 and PRV 161 survived 55 and 50 h, respectively. Bars for A, D, and G, 500 µm; bars for B, E, and H, 50 µm; bars for C, F, and I, 100 µm.

Virulence of PRV 160 and PRV 161 in the rat eye model. Viruses with gE and gI deleted not only have a defect in anterograde spread to the DGN and the SC but also are markedly lessvirulent in rats than the wild-type virus, PRV Becker, as measuredby reduced symptoms of infection and delayed mean time to death(11, 45). Typical symptoms of PRV disease in the rat includeruffling of the fur, nasal discharge, hunched posture, laboredbreathing, uncoordinated movement, and scratching and rubbingof the face, particularly in the area surrounding the injectedeye. These symptoms appear more rapidly after wild-type virusinfection and are much more severe by comparison. In contrast,animals infected with mutant viruses lacking the gE or gI geneslive longer and exhibit milder symptoms, which are delayed inonset. We found that animals infected with Us9 mutants also livedsignificantly longer (Table 2) and exhibited delayed, mildersymptoms. After infection with PRV Becker, the mean time to deathwas 66.9 h (n = 2) and severe symptoms appeared on average asearly as early as 62 h. For animals infected with PRV 91 (gE null)the mean time to death was 88.3 ± 16.1 h and symptoms appearedon average as early as 82 h but were very mild. For animals infectedwith PRV 160, the mean time to death was 96.8 ± 12.9 h and mildsymptoms appeared on average as early as 93 h. For animals infectedwith PRV 161, the mean time to death was approximately 79.2 ±8.5 h and mild symptoms appeared on average as early as 77 h.Animals infected with the revertant viruses PRV 160R or PRV 161Rhad mean times to death of 72.4 and 69.5 h, respectively. Theseanimals also experienced the rapid and severe symptoms typicalfor animals infected with wild-type virus. Wild-type virulencewas also restored in coinfection experiments of PRV 161 and eitherPRV 91 or PRV 98 (data notshown).

Virulence of PRV 160 and PRV 161 in the PFC injection model. When wild-type PRV is injected directly into the PFC, animals rapidly develop severe symptoms and rarely survive longer than48 h (9). In contrast, when PRV Bartha is injected similarly,animals survive to at least 65 h postinfection with only mildsymptoms at time of death. PRV gE and gI null mutants producesomewhat extended times to death compared to wild-type virus,but both PRV Us9 null mutants were as virulent as wild-type virusin this model (Fig. 6). Animals injected with either of the Us9null mutants exhibited a rapid onset of symptoms as they approached48 h of survival and died shortly thereafter. However, in bothinstances the progression to death following the appearance ofsymptoms was very rapid and animals rarely lived beyond 55h.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The lipid envelope of PRV virions contains at least 16 virally encoded membrane proteins (gB, gC, gD, gE, gI, gH, gK, gL,gM, gN, Us9, UL3, UL11, UL20, UL34, and UL43) (28). Among theseenvelope proteins, at least six have been shown to be nonessentialfor growth in tissue culture (28) and are therefore believedto play important roles in the pathogenesis and spread of thevirus in vivo. We have previously identified the protein productof one of these non-essential PRV genes, the Us9 gene, to be a98-amino-acid, phosphorylated membrane protein which is insertedinto the viral envelope in a unique type II tail-anchored topology(5). In such a topology, PRV Us9 is predicted to have a 68-amino-acidcytoplasmic tail and a 3-amino-acid ectodomain. PRV Us9 localizesto the trans-Golgi network region in both infected and transfectedcells and is maintained in this compartment by endocytosis fromthe plasma membrane (6). In this study, we constructed twoUs9 null viruses and examined their growth properties in vitroand invivo.

Neither PRV 160 nor PRV 161 has obvious defects associated with the loss of Us9 in vitro. The Us9 null viruses are indistinguishablefrom wild-type PRV Becker in single-step growth release and plaquesize. Moreover, there is no defect with Us9 null viruses in theexpression, processing, or intracellular localization (data notshown) of the gE, gI, gB, or gC envelope proteins. Nor does theremoval of Us9 from the viral particle affect the incorporationof other viral glycoproteins into the virionenvelope.

We next assessed the contribution of Us9 to transneuronal infection following either intravitreal or intracranial infection.Upon direct infection of the retina, PRV 160 and PRV 161 bothexhibited an anterograde neuronal spread defect. In this model,both Us9 null viruses were defective in anterograde spread tovisual centers involved in visual perception and reflex movementof the eyes, but replicated efficiently in retinal ganglion cellsand their target neurons that are involved in biological timing.Interestingly, the pattern of central infection that is producedby PRV 160 or PRV 161 is indistinguishable from that observedin animals infected with either a gE or gI null virus. The restorationof wild-type spread to all retinorecipient areas following infectionwith the revertant viruses PRV 160R and PRV 161R indicated thatthe neuronal spread defect of PRV 160 and PRV 161 is due to theloss of Us9 and not to additional mutations. This was also supportedby sequencing analysis and mixed-infection experiments with aUs9 null virus and either a gE or gI null virus. A defect in anterogradetransynaptic infection was also observed after injection of gE,gI, or Us9 null mutants into the PFC. In prior work we had demonstratedthat PRV Becker had the capacity to produce an anterograde transynapticinfection of striatal neurons and further showed that this abilitywas lacking in rats injected with the attenuated PRV Bartha strain.The data presented in this report strongly suggests that the inabilityof PRV Bartha to produce an anterograde transynaptic infectionthrough cortical projections to the striatum is related, at leastin part, to the absence to the gE, gI, and Us9 genes from theunique short region of the genome. Interestingly, all of the nullmutations reduced the magnitude of anterograde infection of thestriatum rather than causing a total block, suggesting that theproducts of these genes function together to increase the efficiencyof anterograde infection. Further study is necessary to determinethe validity of thishypothesis.

We also examined the contribution of Us9 to virulence in both the rat eye and PFC models. As observed for gE and gI null viruses,the mean time to death of animals infected with either PRV 160or PRV 161 was extended following intravitreal injection comparedto that due to the wild-type controls. Not only did animals injectedwith the Us9 null viruses live longer than PRV Becker-infectedanimals, they also displayed less-severe symptoms. In contrast,Us9 null mutants were as virulent as wild-type virus after corticalinjection. Further work, however, is necessary to understand theseresults, as gE and gI null viruses are markedly attenuated inthis model. It is noteworthy that a similar differential expressionof virulence was observed with an HSV-1 mutant lacking Us9, Us10,Us11, and Us12 following peripheral or central infection (32).

In this report, we show that the Us9 protein, in addition to the gE and gI glycoproteins, is necessary but not sufficientfor anterograde spread between some, but not all, synapticallyconnected neurons in two models of PRV invasiveness. Althoughmixed-infection experiments in the rat eye model suggest thatall three PRV envelope proteins function at a step after entryof the virus into the primary retinal ganglion cell, several observationsindicate that Us9 may play a role different from that of gE orgI in promoting anterograde spread. The first observation is thatboth gE and gI have been shown to form a heterodimer shortly aftersynthesis in the endoplasmic reticulum (45, 47, 48), andit is often believed that this complex is the functional unitinvolved in transneuronal spread. However, Us9 does not appearto form a complex with either gE or gI. By standard coimmunoprecipitationexperiments, we cannot detect any physical interaction betweenUs9 and the gE-gI complex in either infected cells or in the viralparticle (unpublished data). Further experiments to confirm thisobservation are in progress, as it is possible that Us9 may interactwith gE or gI either transiently or only under certain conditions.The second observation is that both the gE and gI proteins inPRV, as well as in other alphaherpesviruses, are required forefficient cell-to-cell spread in a variety of tissue culture celllines (2, 20, 21, 23, 24, 47). In contrast, thereis no dependence of Us9 on cell-to-cell spread as determined byplaque formation in tissue culture cells. Us9 null viruses formwild-type-sized plaques in all cell lines examined. To accountfor these observations, we propose a model in which the gE-gIcomplex is part of the machinery promoting the spread of virusfrom the presynaptic axon terminal to the postsynaptic cell. Theseproteins are likely to act at the site of egress and need notbe in virus envelopes to promote spread between synaptically connectedneurons, as shown by Tirabassi et al. (42). Accordingly, wesuggest that the gE-gI complex mediates spread through the interactionof the gE-gI ectodomains with a cellular receptor on the postsynapticcell. Interaction of the gE-gI complex with this putative receptorwould be necessary for entry into secondary neurons in the DGNor SC as spread to the retinorecipient circadian areas is gE-gIindependent. A similar model involving the interaction of gE-gIwith a cellular ligand has been recently proposed by Dingwelland Johnson for the spread of HSV-1 between epithelial cells (13).Yet the question remains as to how Us9 promotes anterograde spreadin this model. It does not seem likely that Us9 has the same roleas gE and gI because a Us9 null virus forms wild-type-sized plaquesin tissue culture. Nor does it seem probable that the three aminoacids that constitute the Us9 ectodomain interact with a receptoron an adjacent cell. Rather, we propose that Us9 serves a transportrole in the infected neuron, perhaps delivering newly envelopedviral particles and/or vesicles containing envelope proteins,such as gE and gI, to the axon terminal. In the absence of Us9,neither the virions nor the glycoprotein vesicles would be efficientlytargeted to the site of egress, thereby leading to a defect intransynaptic spread. In support of this idea, Us9 has a topologysimilar to that of proteins involved in vesicular transport, andwe have identified several motifs in the Us9 cytoplasmic tailthat are important for intracellular trafficking (5, 6).We are currently examining viral mutants defective in Us9 intracellulartrafficking to see what effects these motifs have on Us9's abilityto promote anterograde spread in the rodent central nervoussystem.

	ACKNOWLEDGMENTS

We gratefully acknowledge the expert technical assistance of J. Goodhouse and Jen-Shew Yen. Plasmid pPH2 was kindly providedby P. Husak. A.D.B. thanks R. Tirabassi and P. Husak for adviceand guidance with the rat eye model as well as the members ofthe Enquist laboratory for careful reading of the manuscript andhelpfulcomments.

A.D.B. was supported by NIH training grant 5T32GM07388. This work was supported by NINDS grant 1RO133506 to L.W.E. and a grantfrom The John D. and Catherine T. MacArthur Foundation ResearchNetwork on Early Experience and Brain Development to J.P.C.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biology, Princeton University, Princeton, NJ 08544. Phone:(609) 258-2415. Fax: (609) 258-1035. E-mail: Lenquist{at}molbiol.princeton.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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43. Wagenaar, F., J. M. A. Pol, B. Peeters, A. L. J. Gielkens, N. de Wind, and T. G. Kimman. 1995. The US3-encoded protein kinase from pseudorabies virus affects egress of virions from the nucleus. J. Gen. Virol. 76:1851-1859[Abstract/Free Full Text].

44. Watson, R. E., Jr., S. J. Wiegand, R. W. Clough, and G. E. Hoffman. 1986. Use of cryoprotectant to maintain long-term peptide immunoreactivity and tissue morphology. Peptides 7:155-159[Medline].

45. Whealy, M. E., J. P. Card, A. K. Robbins, J. R. Dubin, H. J. Rziha, and L. W. Enquist. 1993. Specific pseudorabies virus infection of the rat visual system requires both gI and gp63 glycoproteins. J. Virol. 67:3786-3797[Abstract/Free Full Text].

46. Zemanick, M. C., P. L. Strick, and R. D. Dix. 1991. Direction of transneuronal transport of herpes simplex virus 1 in the primate motor system is strain-dependent. Proc. Natl. Acad. Sci. USA 88:8048-8051[Abstract/Free Full Text].

47. Zsak, L., F. Zuckermann, N. Sugg, and T. Ben-Porat. 1992. Glycoprotein gI of pseudorabies virus promotes cell fusion and spread via direct cell-to-cell transmission. J. Virol. 66:2316-2325[Abstract/Free Full Text].

48. Zuckermann, F. A., T. C. Mettenleiter, C. Schreurs, N. Sugg, and T. Ben-Porat. 1988. Complex between glycoproteins gI and gp63 of pseudorabies virus: its effect on virus replication. J. Virol. 62:4622-4626[Abstract/Free Full Text].

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46.	Zemanick, M. C., P. L. Strick, and R. D. Dix. 1991. Direction of transneuronal transport of herpes simplex virus 1 in the primate motor system is strain-dependent. Proc. Natl. Acad. Sci. USA 88:8048-8051[Abstract/Free Full Text].
47.	Zsak, L., F. Zuckermann, N. Sugg, and T. Ben-Porat. 1992. Glycoprotein gI of pseudorabies virus promotes cell fusion and spread via direct cell-to-cell transmission. J. Virol. 66:2316-2325[Abstract/Free Full Text].
48.	Zuckermann, F. A., T. C. Mettenleiter, C. Schreurs, N. Sugg, and T. Ben-Porat. 1988. Complex between glycoproteins gI and gp63 of pseudorabies virus: its effect on virus replication. J. Virol. 62:4622-4626[Abstract/Free Full Text].