Membrane Targeting Properties of a Herpesvirus Tegument Protein-Retrovirus Gag Chimera

doi:10.1128/JVI.74.18.8692-8699.2000

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Journal of Virology, September 2000, p. 8692-8699, Vol. 74, No. 18
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Membrane Targeting Properties of a Herpesvirus Tegument Protein-Retrovirus Gag Chimera

J. Bradford Bowzard, Robert J. Visalli, Carol B. Wilson, Joshua S. Loomis, Eric M. Callahan, Richard J. Courtney, and John W. Wills^*

Department of Microbiology and Immunology, The Pennsylvania State University College of Medicine, Hershey, Pennsylvania 17033

Received 8 December 1999/Accepted 26 June 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The retroviral Gag protein is capable of directing the production and release of virus-like particles in the absence of allother viral components. Budding normally occurs after Gag is transportedto the plasma membrane by its membrane-targeting and -binding(M) domain. In the Rous sarcoma virus (RSV) Gag protein, the Mdomain is contained within the first 86 amino acids. When M isdeleted, membrane association and budding fail to occur. Buddingis restored when M is replaced with foreign membrane-binding sequences,such as that of the Src oncoprotein. Moreover, the RSV M domainis capable of targeting heterologous proteins to the plasma membrane.Although the solution structure of the RSV M domain has been determined,the mechanism by which M specifically targets Gag to the plasmamembrane rather than to one or more of the large number of internalmembrane surfaces (e.g., the Golgi apparatus, endoplasmic reticulum,and nuclear, mitochondrial, or lysosomal membranes) is unknown.To further investigate the requirements for targeting proteinsto discrete cellular locations, we have replaced the M domainof RSV with the product of the unique long region 11 (U_L11) geneof herpes simplex virus type 1. This 96-amino-acid myristylatedprotein is thought to be involved in virion transport and envelopmentat internal membrane sites. When the first 100 amino acids ofRSV Gag (including the M domain) were replaced by the entire UL11sequence, the chimeric protein localized at and budded into theGolgi apparatus rather than being targeted to the plasma membrane.Myristate was found to be required for this specific targeting,as were the first 49 amino acids of UL11, which contain an acidiccluster motif. In addition to shedding new light on UL11, theseexperiments demonstrate that RSV Gag can be directed to internalcellular membranes and suggest that regions outside of the M domaindo not contain a dominant plasma membrane-targetingmotif.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Although viruses use a variety of different replication strategies, one step common to all of these pathways is the accumulationof virion components at a specific location within the cell toform new infectious particles. To efficiently arrive at the designatedsite of assembly, viral proteins contain specific targeting signals.Retroviruses are useful for investigating these targeting signalsbecause budding is directed by a single, well-studied viral proteinnamed Gag (Fig. 1).

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FIG. 1. UL11-Gag chimeras. The wild-type RSV Gag (unshaded) and UL11 (hatched) proteins are aligned at their N termini. The positions of the assembly domains are marked along the top of Gag. Sites cleaved by the viral protease are marked by vertical lines through Gag. N-terminal myristylation is indicated by a squiggled line. Numbers indicate the amino acids included in each construct. The p6 sequence of HIV, the first 10 amino acids of the Src oncoprotein, and the GFP sequences are indicated by black boxes.

Gag proteins are synthesized on free ribosomes and subsequently transported and assembled into particles on the cytoplasmicface of the plasma membrane. Only three small modular regionsof Gag (termed assembly domains) are required for particle formation(39). The interaction (I) domain within the nucleocapsid (NC)region facilitates the formation of the Gag-Gag contacts necessaryfor the production of dense particles (3, 6, 43). Themembrane-targeting and -binding (M) domain is responsible fordirecting Gag from the cytoplasm to the plasma membrane (21,40, 47). Once at the plasma membrane, the late (L) domaincoordinates the final release of the particle from the cell surface(14, 22, 45). At this time, Gag is cleaved by the viralprotease to generate the mature viral proteins (MA, p2, p10, CA,NC, PR; J. W. Wills and R. C. Craven, Editorial, AIDS 5:639-654,1991) (Fig. 1).

Although Gag is normally directed to the plasma membrane, proteins from some other viruses concentrate at different membranesites. For example, herpes simplex virus type 1 (HSV-1) expressesa 96-amino-acid protein from the U_L11 gene (18) (here referredto as the UL11 protein) (Fig. 1) that appears to be targeted toperinuclear membranes (1). Because Gag and UL11 localize todistinct cellular locations, it is likely that they use differenttargetingsignals.

The targeting signals of Gag have been extensively studied. The retroviral M domain is contained within the matrix (MA) sequenceat the amino terminus of Gag (Fig. 1). Positively charged aminoacids are important features of the Rous sarcoma virus (RSV) andhuman immunodeficiency virus (HIV) M domains (23, 50), asis myristate for the M domains of HIV, murine leukemia virus,and Mason-Pfizer monkey virus (7, 15, 29, 30, 38).M is required for plasma membrane localization, and disruptionof its amino terminus abrogates budding and results in Gag remainingcytoplasmic (7, 38, 47). In addition, M alone is sufficientto target heterologous cytoplasmic proteins to the plasma membrane(40, 50).

Despite its importance for plasma membrane localization, it is not entirely clear that the M domain is the sole targetingdeterminant within Gag. For example, cleavage of Gag during retroviralparticle maturation releases MA from the rest of the protein.Upon entry of the mature particle into a host cell, some of thisfree MA no longer associates with the plasma membrane, even thoughit contains the intact M domain (8, 16, 28). Why is theM domain inactive in this context? It is possible that cleavageof MA from the remainder of Gag allows conformational rearrangementsthat disrupt the M domain and prevent plasma membrane binding(37, 50). An alternate explanation is that sequences in regionsof Gag other than MA affect localization in some way, either byproviding additional targeting information that is required fortransport to the plasma membrane or by providing cooperativityto strengthen the avidity of the membrane-binding domain. Aftercleavage of MA, these secondary signals would no longer be availableto promote plasma membrane association. To address this issue,we replaced the M domain of RSV with the UL11 protein from HSV-1.Our results show that UL11-Gag chimeras localized to internalmembranes (like UL11 alone) rather than to the plasma membrane,suggesting that the C terminus of Gag does not contain dominantplasma membrane-targeting signals. These experiments also revealedsome of the sequence elements required for UL11-directed membranebinding and provided reagents for further investigation of therole of UL11 in herpesvirusassembly.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Previously constructed gag alleles. The RSV gag gene was obtained from pATV-8, an infectious molecular clone of the Prague C genome (34). The HSV-1 U_L11 genewas amplified from the KOS strain (35). The plasmid pSV.Myr1used in these experiments has been described previously (46).Standard protocols were used for all DNA manipulations (31),and all plasmids were propagated in Escherichia coli DH-1 cellsin 2× YT medium containing 25 µg of ampicillin per ml, with theexception of the green fluorescent protein (GFP) vectors, whichwere propagated in the presence of 50 µg of kanamycin perml.

Newly constructed gag alleles. Several Gag chimeras were made to replace the RSV M domain with various portions of the UL11 protein of HSV-1. For the herpesvirus-myristylatedGag (HMG) construct, the entire UL11 coding sequence was obtainedby PCR amplification from the KOS genome with a forward primerthat was complementary to the HSV sequence located 100 bases upstreamof the initiator ATG and a reverse primer complementary to thesequence coding for the final five amino acids of UL11. The 5'ends of the primers also contained recognition sites for the SstI(forward) and SpeI (reverse) restriction endonucleases (underlined).After amplification with these primers (forward, 5'-ACCAGGCCGTTGAGCTCGCCCTGATCATTA-3';reverse, 5'-CATTGTTTTGGTACTAGTTCGCTATCGGACAT-3'), the productwas digested with SstI and SpeI and ligated to the large fragmentgenerated by digesting pSV. $Delta$ MA6S (21) with SstI and SpeI. Theresulting plasmid was named pSV.HMG. The constructs in which N-terminalfragments of UL11 were fused to Gag were also made by PCR withthe forward primer listed above in combination with reverse primersthat contained an SpeI site (underlined) and that were complementaryto internal UL11 sequences (ending at codon 70 [5'-TGAGTGTGGCGCACTAGTGGGTCCGAT-3'],codon 49 [5'-CCCGCGCATATCCACTAGTACGTAGAAAT-3'], or codon 23 [5'-GCGAGACGACCACTAGTTCGTCGGTGAT-3').The resulting plasmids were named pSV.HMG.70, pSV.HMG.49, andpSV.HMG.23,respectively.

A mutant encoding a myristate-minus form of HMG was produced by combining the products of two PCR fragments before cloningwith the SstI and SpeI sites. The "left" fragment was amplifiedby using the HMG forward primer and a reverse primer that wascomplementary to the region flanking the UL11 initiator ATG. Thisreverse primer (5'-GAGAGGCCCATATGTCGGCGAGCGT-3') retains the ATG,but contains two changes that create an overlapping NdeI site(underlined). The PCR mixture for the "right" fragment used theoriginal HMG reverse primer and a forward primer that containstwo mismatches to create an NdeI site (underlined) at the sameposition mentioned above. This forward primer (5'-GCTCGCCGACATATGG <UNL>C</UNL>

CCTCTCGTTCT-3')also contains an additional mismatch (double underlined) thatchanges the second UL11 codon (glycine) to one for alanine. Thetwo amplified products were digested with NdeI, ligated together,and reamplified with the forward primer used to make the lefthalf and the reverse primer used to make the right half. Thisproduct was digested with SstI and SpeI and cloned into pSV. $Delta$ MA6Sto create pSV.HM( $-$ )G.

pSV.Src.HMG was made by a similar strategy. For this construct, the left fragment was amplified with pSV.Myr1 as the templateand upstream and downstream primers completely complementary topSV.Myr1 sequences flanking the SstI (nucleotide [nt] 255) andMluI (nt 408) sites, respectively. The right fragment was amplifiedfrom pSV.HMG template DNA with a forward primer (5'-ACGCTCGCCACGCG <UNL>T</UNL>

TGGGCCTCTCGTT-3')containing an MluI site which overlaps a mismatch (double underlined)that changes the first base of the start codon from an A to aT. The left and right fragments were digested with MluI, ligatedtogether, and reamplified as described above. The resulting fragmentwas digested with SstI and SpeI and ligated to the large fragmentgenerated by digesting pSV. $Delta$ MA6S with SstI and SpeI.

The protease (PR)-coding region was deleted from pSV.HMG by digesting pSV.Myr1.3h (42) with KpnI and SstII and ligatingthe large fragment to the small fragment produced by digestingpSV.HMG with KpnI and SstII. The resulting PR mutant was namedpSV.HMG.3h. To create pSV.HMG.p6, the large fragment generatedby digesting pSV.T10C.p6 (22) with SstI and BlpI was ligatedto the small fragment generated by digesting pSV.HMG with thesameenzymes.

GFP-containing constructs were made after cloning Gag-coding sequences into the Clontech pEGFP-N2 vector. To do this, oligonucleotide-directedM13 mutagenesis of the wild-type gag gene (46) was used to createan ApaI site (underlined) near the junction of the NC- and PR-codingsequences (5'-TCGGGGCCGTGGCCCGGGCCCGAGCCACCTGCCGTCTCG-3'). Gagsequences were removed from replicative form DNA by SstI-ApaIdigestion and placed in frame into the Clontech vector to formpGag.GFP. To create pHMG.GFP, which encoded a GFP-tagged formof the UL11-Gag chimera, the small fragment from an SstI-EspIdigest of pSV.HMG was purified and ligated to the large fragmentfrom an SstI-EspI digest of pGag.GFP. pHM( $-$ )G.GFP was generatedby the same procedure, but the small fragment was obtained frompSV.HM( $-$ )G. To create pUL11.GFP, the UL11 coding sequence wasamplified with the same forward primer that was used to createHMG. The reverse primer (5'-TCAGGAATTCGCTATCGGA-3') was complementaryto the coding sequence of the C terminus of UL11 and had a noncomplementaryregion that contained an EcoRI site (underlined). This productwas digested with SstI and EcoRI and ligated to the large fragmentgenerated by digestion of pEGFP-N2 with the sameenzymes.

To enable transient and stable expression in QT6 avian cells, UL11-coding sequences were transferred into an RSV proviralvector that contains the hygromycin resistance gene. pRC.HMG wasconstructed by ligating the large fragment generated by digestingthe BHRCAN vector (12) with SstI and HpaI to the small fragmentgenerated by digesting pSV.HMG with BssHII, treating it, withKlenow fragment, and digesting it with SstI.

Transfection and labeling of cells and immunoprecipitation of Gag proteins. COS-1 cells were transfected by the DEAE-dextran-chloroquine method, as previously described (46). Approximately 48 h aftertransfection, the cells were labeled for either 5 min or 2.5 hwith 50 µCi (>1,000 Ci/mmol) of L-[³⁵S]methionine. The cells and growth medium from each labeled culturewere separated and mixed with lysis buffer containing proteaseinhibitors (46). The Gag proteins were immunoprecipitated withpolyclonal rabbit serum against whole RSV (reacts with MA, CA,NC, and PR [42]). The immunoprecipitated proteins were resolvedby electrophoresis in sodium dodecyl sulfate-12% polyacrylamidegels and detected by fluorograpy (46). QT6 cells were transfectedby the calcium phosphate transfection method as previously described(12).

Budding efficiency was determined by first calculating, for each construct, the ratio of protein released into the mediumduring a 2.5-h labeling to the amount made in the lysates duringa 5-min pulse. The ratio of each mutant was divided by the ratioof the wild type to yield its relative buddingefficiency.

Immunofluorescence and confocal and electron microscopy. Cells were transfected as described above for all microscopic analyses. For immunofluorescence, cells were fixed with 5% aceticacid-95% ethanol at $-$ 20°C (48), blocked with 0.1% rabbit serumalbumin in phosphate-buffered saline, and incubated with rabbitanti-RSV polyclonal primary antibodies (42) and goat anti-rabbitsecondary antibodies conjugated to either fluorescein isothiocyanate(FITC) or tetramethyl rhodamine isothiocyanate (TRITC) (Sigma).The procedure for double-label immunofluorescence was the sameas that described above, except that the primary antibody wasa mixture of the anti-RSV polyclonal antibody and a mouse anti-Golgi58-kDa protein (Sigma) and the secondary antibody was a mixtureof goat anti-rabbit immunoglobulin G conjugated to TRITC and goatanti-mouse immunoglobulin G conjugated to FITC (Sigma). Cellswere visualized by light microscopy and a filter set appropriatefor the fluorescent label, and images were captured on Kodak T400black and white photographic film. Confocal microscopy was donewith a Zeiss LSM microscope, and the captured images were coloredand digitally combined in Adobe Photoshop. For electron microscopy,transfected cells were grown in Permanox plates, fixed with glutaraldehyde-paraformaldehyde,postfixed in osmium-potassium ferrocyanide, dehydrated throughincreasing concentrations of ethanol, and embedded in Epon 812(11). Thin sections were stained with uranyl acetate-lead citrateand viewed on a Phillips 400 electronmicroscope.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

To investigate the role of sequences other than the M domain in plasma membrane targeting, we replaced the first 100 aminoacids of RSV Gag with a heterologous membrane-binding sequence.Because its size approximates that of the M domain (96 versus86 amino acids, respectively) and it is localized to internalmembranes, the myristylated herpesvirus protein UL11 was used(Fig. 1). If the M domain is the only source of targeting informationwithin wild-type Gag, then the localization of the UL11-Gag chimera(HMG; Fig. 1) should be similar to that of UL11 alone (i.e., atinternal membranes). If Gag sequences outside the M domain promoteplasma membrane targeting, then the localization of HMG mightbe similar to that of full-length Gag or at least different fromthat ofUL11.

The UL11-RSV Gag chimera HMG is budding deficient. Since Gag can mediate budding when it is localized to the plasma membrane by a heterologous signal (47), particle releasewas initially monitored as a marker for plasma membrane targeting.When two clones of HMG were expressed in COS-1 cells (Fig. 2),a precursor protein of the expected size (~76 kDa) was observedin the cell lysates along with the CA and PR Gag cleavage products(4, 11, 46). Although the efficient proteolytic processingof the Gag precursor seen here is indicative of membrane binding(46, 47), it was also noted that the CA in the HMG lanes wasnot further processed to form the characteristic triplet of bands.This phenotype has previously been associated with RSV Gag mutantsthat do not bud (47), so it was not surprising that no Gag products(and hence no virus-like particles) from either of the two HMGclones were visible in the extracellular medium (Fig. 2, comparelanes 1 and 2 with lane 3). It is important to note that the lackof budding is not caused by the lack of CA processing, since PR-deficientmutants as well as Gag proteins engineered to produce only thelower CA species bud efficiently (46, 49).

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FIG. 2. Expression of HMG. COS-1 cells transfected with the indicated constructs were labeled for 2.5 h with L-[³⁵S]methionine, and the Gag proteins from the media and cell lysates were immunoprecipitated with anti-RSV antibodies, separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, and visualized by autoradiography. The numbers to the left are the positions (in kilodaltons) of molecular mass markers. The positions of the CA and PR Gag cleavage products are also indicated. Gag products in the medium are indicative of budding.

Since these findings suggest that HMG is membrane bound, the lack of budding is consistent with HMG being localized to a membraneother than the plasma membrane. However, the lack of budding isa negative result, and there are ways that particle release couldbe inhibited even if HMG was located at the plasma membrane. Forexample, if the viral PR is more active than usual in the contextof HMG, then the UL11-Gag molecules would be cleaved before theyare able to complete the budding process (9). This would causethe nascent buds to collapse back into the cytoplasm and resultin the observed lack-of-budding phenotype. Since PR is not requiredfor budding, 90% of it was deleted to form HMG.3h (Fig. 1). Thischimera was neither cleaved nor released into the medium (Fig.3, lanes 6), indicating that HMG is not budding deficient becauseof enhanced PR activity.

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FIG. 3. Release properties of modified forms of HMG. The indicated constructs were transfected into duplicate plates of COS-1 cells. The right panel (media) was from one set of plates that were treated as described in the legend to Fig. 2. Gag proteins in the left panel (lysates) were collected and visualized as for Fig. 2, but were from the second set of plates that had been labeled for only 5 min.

Another way that HMG might be blocked for budding even if it had been directed to the plasma membrane is by interference withthe nearby L domain (Fig. 1), which is required for the virus-cellseparation step (45). L domain mutants are targeted to the plasmamembrane and, like HMG, undergo proteolytic processing, but donot bud. Previous experiments have shown that budding can be restoredto RSV L domain mutants by the addition of the HIV p6 sequence,which also contains an L domain (22), and with this in mind,HMG.p6 was constructed (Fig. 1). Although it was expressed well(Fig. 3, lane 4, lysates), none of the protein was released intothe medium. Thus, it appears unlikely that an L domain defectcaused the retention of HMG inside thecell.

A third possibility to explain the failure of HMG to be released after being targeted to the plasma membrane is that the UL11sequences are bulky and inhibit the budding process. To test thisidea, the strong plasma membrane-binding domain of the Src oncoproteinwas attached to the amino terminus of HMG to create Src.HMG (Fig.1). If HMG is already at the plasma membrane and is preventedfrom budding by the UL11 sequences, then this modification shouldhave no effect. However, if HMG is directed to an internal membrane,then release into the culture medium might be restored. We foundthat Src.HMG was released into the medium (Fig. 3, lanes 7; 40%efficiency relative to the wild type), indicating that the UL11sequences are not incompatible with budding and further supportingthe idea that the L domain within HMG isintact.

An additional possibility to explain the failure of HMG to be released is that it is not bound to any membrane at all. IfHMG is partitioned into the cytoplasm, then it might be packagedinto particles when coexpressed with wild-type Gag molecules.However, unlike membrane-binding mutants of RSV (5, 47),HMG was not detectably rescued (data not shown). Although thisis a negative result, it is consistent with a rapid transportof HMG to an internal-membranelocation.

HMG is targeted to the Golgi apparatus. In an attempt to gather direct evidence that HMG is localized to a membrane other than the plasma membrane, immunofluorescenceanalysis was performed. Expression of full-length RSV Gag in COScells, followed by fixation and staining, revealed a diffuse fluorescencethroughout the cell (Fig. 4A). In contrast, similar analyses withHMG showed a distinct staining pattern in a tight juxtanuclearlocation (Fig. 4B). To identify the cellular compartment containingHMG, double-label immunofluorescence and confocal microscopy wereused. A 1-µm optical slice of a single transfected cell labeledwith antibodies against RSV (Fig. 4D) and against the Golgi 58-kDaprotein (58K) (Fig. 4E) shows colocalization of HMG and the Golgiapparatus-specific marker (Fig. 4F).

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FIG. 4. Microscopic analyses of HMG-expressing cells. COS-1 cells were transfected with the indicated constructs. Cells in panels A to F were analyzed by immunofluorescence. In panels A to C, antibodies specific for RSV Gag were used. Cells in panels D to F were double labeled with a mixture of rabbit antibodies against Gag and mouse antibodies against the Golgi 58K protein, which were detected by using a mixture of goat anti-rabbit antibodies conjugated to TRITC and goat anti-mouse antibodies conjugated to FITC. Panels D and E are the same field viewed by confocal microscopy with the appropriate wavelength to excite TRITC (D) or FITC (E) and were digitally combined to provide the image in panel F. Cells transfected with GFP constructs in panels G and H were viewed by light microscopy without fixing or staining. Cells in panels I and J were analyzed by standard electron microscopy.

Although it is clear that HMG is localized to the Golgi apparatus within fixed cells, it was possible that the chemical permeabilizationand fixation processes might have altered the normal cellulardistribution of HMG (20). To completely rule out this possibility,GFP was fused to the C terminus of HMG, and the localization ofthe resulting chimera (HMG.GFP; Fig. 1) was visualized in livingcells. HMG.GFP appeared to be exclusively perinuclear (Fig. 4G),indicating that the Golgi apparatus targeting observed by immunofluorescencewas not a fixation artifact. To assess whether the Gag sequencesof HMG contribute to the Golgi apparatus targeting, UL11 was fuseddirectly to either GFP (UL11.GFP; Fig. 1) or the nine-amino-acidhemagglutinin (HA) tag. The localization of UL11.GFP (Fig. 4H)and UL11.HA (data not shown) was identical to that of HMG.GFP,suggesting that UL11 alone is able to travel to and bind Golgimembranes.

To determine whether HMG merely binds to the cytoplasmic face of the Golgi membranes or whether interactions among the Gagportion of the chimera also mediate budding into the Golgi cisternae,electron microscopy was employed to achieve increased resolution.In contrast to untransfected COS-1 cells (not shown), normal Golgistacks were not observed (Fig. 4I and J). Instead, thickened,electron-dense membranes similar in appearance to budding retroviruseswere observed in the same perinuclear location that was fluorescentlylabeled, but they were not seen at the plasma membrane. Due tothe substantial disruption of the Golgi compartment, it is notclear whether virus-like particles are released into the cisternae.However, because membrane distortion is required during Gag-mediatedbudding and because HMG is capable of directing budding when targetedto the plasma membrane with the Src membrane-binding domain, thisresult is consistent with internalbudding.

Requirements for Golgi targeting by UL11. Many (but not all) myristylated proteins require the addition of myristate for proper targeting and/or membrane binding. Todetermine whether this requirement exists for HMG, we constructeda myristate-negative form of HMG (Fig. 1). Although HM( $-$ )G wasexpressed well, it was not released into the medium (Fig. 3, lanes5), and immunofluorescence analysis showed diffuse cytoplasmicstaining (Fig. 4C). The lack of perinuclear staining indicatesthat myristylation is required for Golgilocalization.

To determine which amino acids are required for Golgi localization, three C-terminal deletions of the UL11 portion of HMGwere made (Fig. 1). Metabolic labeling of the deletion mutantsshowed protein production and processing, but little (HMG.23;Fig. 5A, lane 4; 7% relative to RSV Gag) or no (HMG.70 and HMG.49;Fig. 5A, lanes 2 and 3, respectively) release into the medium.By immunofluorescence, HMG.70 and HMG.49 show strong Golgi staining,while HMG.23 shows cytoplasmic staining in addition to weak Golgistaining (Fig. 5B). The significant intracellular cleavage ofHMG.23, as well as the increased amount of budding by this protein(Fig. 5A, lanes 4), indicates that it is directed to the plasmamembrane to some extent. Thus, the Golgi apparatus-specific targetingsignal is contained entirely within the first 49 but not the first23 amino acids of UL11. Taken together, these data suggest thatthe first 23 residues of UL11 contain a nonspecific membrane-bindingfunction that is affected by the information contained withinresidues 24 to 49.

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FIG. 5. Deletion analysis of UL11. (A) The level of particle release of the indicated mutants was measured by labeling the transfected cells as in Fig. 3. (B) COS-1 cells were transfected, fixed, and stained with RSV Gag-specific antibodies and visualized by confocal microscopy.

The efficiency of Golgi targeting was found to be cell type dependent. In contrast to the lack of budding from COS-1 cells(Fig. 2 and 3), HMG is able to escape from QT6 avian cells with40% the efficiency of RSV Gag (Fig. 6A, lanes 1 and 2 versus lanes3), suggesting some degree of plasma membrane targeting. Thisdifferential targeting is not due to the Gag portion of the chimera,since the localization of UL11.GFP (which contains no Gag sequences)is exclusively perinuclear in mammalian cells (COS-1; Fig. 4 and6B; BHK, Vero, and human melanoma cells [data not shown]), butshows both perinuclear and plasma membrane staining in QT6 cells(Fig. 6B). These data raise the possibility that membrane localizationis influenced by cellular factors that are divergent between mammalianand avian cells and that these factors may play a role in herpesvirusinfections.

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FIG. 6. Expression of HMG in avian cells. The HMG and RSV Gag genes were transferred into the BHRCAN (12) vector for expression in avian cells. (A) Plasmids were transfected by the calcium-phosphate precipitation method into QT6 cells, and the proteins were labeled and collected as described in the legend to Fig. 2. (B) COS-1 or QT6 cells were transfected as for panel A with either GFP or UL11.GFP and viewed by confocal microscopy.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Role of RSV Gag C terminus in plasma membrane localization. By redirecting a UL11-RSV Gag chimera to the Golgi apparatus, our current experiments have provided evidence that the C terminusof Gag does not contain dominant plasma membrane targeting sequences.However, the efficiency of membrane localization of both HIV andRSV Gag is affected by sequences downstream of the amino-terminalM domain (27, 47). These downstream sequences may influencemembrane localization by enhancing the ability of Gag to remainbound at its destination after arrival. One way to increase theavidity of the M domain-membrane interaction is by linking largenumbers of Gag proteins together. Since the I domains are foundwithin NC and are involved in Gag multimerization (39), theyare likely mediators of the C-terminal sequence contribution toGag localization (32).

Another way in which the Gag C terminus may increase the efficiency of membrane localization is by facilitating the transportof Gag from the cytoplasm to the destination specified by theM domain. Trafficking of both cellular (10) and viral (13,36) components can be accomplished by interaction with the microtubuleand microfilament elements of the cytoskeletal transport network.Therefore, the colocalization of Gag with actin in infected cells(24, 25) and the binding of NC within the virion to actin(17, 44) suggest that an interaction of the C terminus ofGag with the cytoskeleton may also play a role in Gagtransport.

Mechanism of UL11 Golgi apparatus targeting. Although it is less than 100 amino acids long, UL11 must contain signals to direct it to and retain it specifically at theGolgi apparatus. Evidence presented here indicates that thesetargeting sequences are contained within the myristylated amino-terminal49 residues. What information is contained in the first 49 residues?When we aligned the UL11 sequences of several herpesviruses, astriking acidic cluster (33) was revealed (Fig. 7, residues37 to 43). Since certain acidic clusters are known to direct proteinsto the trans-Golgi network (TGN) via an association with the PACS-1protein (41), it is possible that UL11 is targeted to the Golgiapparatus in a similar manner. Indeed, the peripheral membraneprotein Nef from HIV-1 has recently been shown to recycle fromthe plasma membrane to the TGN via a PACS-1-dependent mechanism(26).

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FIG. 7. Alignment of UL11 homologs. The amino acid sequences of the UL11 homologs from several herpesviruses are shown. HHV, human herpesvirus. Identical amino acids are indicated by an asterisk, while similar amino acids are marked by a colon. A conserved acidic cluster motif is underlined.

The role of myristylation in UL11 localization is also unclear. The loss of Golgi apparatus targeting of HM( $-$ )G is presumablydue to the loss of membrane binding, rather than a loss of targeting,since nonspecific binding (as was seen for HMG.23) was not observed.However, we cannot rule out the possibility that myristate isrequired for UL11 to associate with a PACS-1-like protein andtherefore is needed for Golgi targeting as well as membranebinding.

Role of UL11 in herpesvirus replication. UL11 is targeted to internal cellular membranes (1) that are identified here as those of the Golgi apparatus. We have alsoshown that this specific localization is independent of all otherviral proteins. However, the role of UL11 at these membranes duringHSV infection remains unclear. UL11 is required for efficientenvelopment and particle release (2, 19), but it is not knownwhether UL11 itself is the primary mediator of the budding event.Our microscopy data indicated severe involution of the internalmembranes. We attributed these effects to the Gag portion of theHMG.GFP protein, but we cannot discount the possibility of a contributionfromUL11.

Another possibility is that UL11 does not drive envelopment but instead recruits other viral proteins to the site of assembly.As a membrane-bound virion protein, UL11 would be ideal as a "bridge"linking the viral envelope to other components of the tegument.These additional tegument proteins, alone or in combination, couldprovide the budding machinery. The amino-terminal halves of UL11homologs from several herpesviruses, which include the targetinginformation, have significant sequence similarity (Fig. 7). Thisis expected for domains that must interface with conserved cellularstructures, such as those of a trafficking pathway. The C terminiof the homologs are more divergent, presumably to accommodatebinding to other viral proteins not conserved between herpesviruses.Experiments to test these models are currently underway.

The assembly pathways of retroviruses and herpesviruses are very different, but they do share the common requirement of targetingthe virion proteins to the correct site of assembly. We have nowdemonstrated that RSV Gag sequences downstream of the M domaindo not contain dominant plasma membrane-specific localizationsignals. We have also identified and partially characterized themembrane-binding and -targeting motif of the HSV-1 UL11 protein.Although further experiments will be needed to dissect the functionalcomponents of the first half of UL11, the information providedhere will be useful in designing these and other investigationsinto the mechanisms of protein targeting and herpesvirusassembly.

	ACKNOWLEDGMENTS

We thank Roland Meyers for performing the thin sectioning and assisting with all aspects of the electronmicroscopy.

This research was sponsored by National Institutes of Health (NIH) grants to R.J.C. (CA42460 and CA60395) and J.W.W. (CA47482).J.B.B. was partially supported by NIH training grant CA60395,and J.S.L. was partially supported by an LSC fellowship from PennsylvaniaStateUniversity.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, Pennsylvania State University College ofMedicine, 500 University Dr., P.O. Box 850, Hershey, PA 17033.Phone: (717) 531-3528. Fax: (717) 531-6522. E-mail: jwills{at}psu.edu.

Present address: Infectious Diseases Section, Wyeth Ayerst Research, Pearl River, NY10965.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Baines, J. D., R. J. Jacob, L. Simmerman, and B. Roizman. 1995. The herpes simplex virus 1 U_L11 proteins are associated with cytoplasmic and nuclear membranes and with nuclear bodies of infected cells. J. Virol. 69:825-833[Abstract/Free Full Text].

2. Baines, J. D., and B. Roizman. 1992. The U_L11 gene of herpes simplex virus 1 encodes a function that facilitates nucleocapsid envelopment and egress from cells. J. Virol. 66:5168-5174[Abstract/Free Full Text].

3. Bennett, R. P., T. D. Nelle, and J. W. Wills. 1993. Functional chimeras of the Rous sarcoma virus and human immunodeficiency virus Gag proteins. J. Virol. 67:6487-6498[Abstract/Free Full Text].

4. Bennett, R. P., S. Rhee, R. C. Craven, E. Hunter, and J. W. Wills. 1991. Amino acids encoded downstream of gag are not required by Rous sarcoma virus protease during Gag-mediated assembly. J. Virol. 65:272-280[Abstract/Free Full Text].

5. Bennett, R. P., and J. W. Wills. 1999. Conditions for copackaging Rous sarcoma virus and murine leukemia virus Gag proteins during retroviral budding. J. Virol. 73:2045-2051[Abstract/Free Full Text].

6. Bowzard, J. B., R. P. Bennett, N. K. Krishna, S. M. Ernst, A. Rein, and J. W. Wills. 1998. Importance of basic residues in the nucleocapsid sequence for retrovirus Gag assembly and complementation rescue. J. Virol. 72:9034-9044[Abstract/Free Full Text].

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1.	Baines, J. D., R. J. Jacob, L. Simmerman, and B. Roizman. 1995. The herpes simplex virus 1 U_L11 proteins are associated with cytoplasmic and nuclear membranes and with nuclear bodies of infected cells. J. Virol. 69:825-833[Abstract/Free Full Text].
2.	Baines, J. D., and B. Roizman. 1992. The U_L11 gene of herpes simplex virus 1 encodes a function that facilitates nucleocapsid envelopment and egress from cells. J. Virol. 66:5168-5174[Abstract/Free Full Text].
3.	Bennett, R. P., T. D. Nelle, and J. W. Wills. 1993. Functional chimeras of the Rous sarcoma virus and human immunodeficiency virus Gag proteins. J. Virol. 67:6487-6498[Abstract/Free Full Text].
4.	Bennett, R. P., S. Rhee, R. C. Craven, E. Hunter, and J. W. Wills. 1991. Amino acids encoded downstream of gag are not required by Rous sarcoma virus protease during Gag-mediated assembly. J. Virol. 65:272-280[Abstract/Free Full Text].
5.	Bennett, R. P., and J. W. Wills. 1999. Conditions for copackaging Rous sarcoma virus and murine leukemia virus Gag proteins during retroviral budding. J. Virol. 73:2045-2051[Abstract/Free Full Text].
6.	Bowzard, J. B., R. P. Bennett, N. K. Krishna, S. M. Ernst, A. Rein, and J. W. Wills. 1998. Importance of basic residues in the nucleocapsid sequence for retrovirus Gag assembly and complementation rescue. J. Virol. 72:9034-9044[Abstract/Free Full Text].
7.	Bryant, M., and L. Ratner. 1990. Myristoylation-dependent replication and assembly of human immunodeficiency virus 1. Proc. Natl. Acad. Sci. USA 87:523-527[Abstract/Free Full Text].
8.	Bukrinsky, M. I., N. Sharova, T. L. McDonald, T. Pushkarskaya, W. G. Tarpley, and M. Stevenson. 1993. Association of integrase, matrix, and reverse transcriptase antigens of human immunodeficiency virus type 1 with viral nucleic acids following acute infection. Proc. Natl. Acad. Sci. USA 90:6125-6129[Abstract/Free Full Text].
9.	Burstein, H., D. Bizub, and A. M. Skalka. 1991. Assembly and processing of avian retroviral gag polyproteins containing linked protease dimers. J. Virol. 65:6165-6172[Abstract/Free Full Text].
10.	Carson, J. H., S. Kwon, and E. Barbarese. 1998. RNA trafficking in myelinating cells. Curr. Opin. Neurobiol. 8:607-612[CrossRef][Medline].
11.	Craven, R. C., A. E. Leure-duPree, C. R. Erdie, C. B. Wilson, and J. W. Wills. 1993. Necessity of the spacer peptide between CA and NC in the Rous sarcoma virus Gag protein. J. Virol. 67:6246-6252[Abstract/Free Full Text].
12.	Craven, R. C., A. E. Leure-duPree, R. A. Weldon, Jr., and J. W. Wills. 1995. Genetic analysis of the major homology region of the Rous sarcoma virus Gag protein. J. Virol. 69:4213-4227[Abstract/Free Full Text].
13.	Cudmore, S., P. Cossart, G. Griffiths, and M. Way. 1995. Actin-based motility of vaccinia virus. Nature 378:636-638[CrossRef][Medline].
14.	Gottlinger, H. G., T. Dorfman, J. G. Sodroski, and W. A. Haseltine. 1991. Effect of mutations affecting the p6 Gag protein on human immunodeficiency virus particle release. Proc. Natl. Acad. Sci. USA 88:3195-3199[Abstract/Free Full Text].
15.	Gottlinger, H. G., J. G. Sodroski, and W. A. Haseltine. 1989. Role of capsid precursor processing and myristoylation in morphogenesis and infectivity of human immunodeficiency virus type 1. Proc. Natl. Acad. Sci. USA 86:5781-5785[Abstract/Free Full Text].
16.	Karageorgos, L., P. Li, and C. Burrell. 1993. Characterization of HIV replication complexes early after cell-to-cell infection. AIDS Res. Hum. Retrovir. 9:817-823[Medline].
17.	Liu, B., R. Dai, C.-J. Tian, L. Dawson, R. J. Gorelick, and X.-F. Yu. 1999. Interaction of the human immunodeficiency virus type 1 nucleocapsid with actin. J. Virol. 73:2901-2908[Abstract/Free Full Text].
18.	MacLean, C. A., B. Clark, and D. J. McGeoch. 1989. Gene UL11 of herpes simplex virus type 1 encodes a virion protein which is myristylated. J. Gen. Virol. 70:3147-3157[Abstract/Free Full Text].
19.	MacLean, C. A., A. Dolan, F. E. Jamieson, and D. J. McGeoch. 1992. The myristylated virion proteins of herpes simplex virus type 1: investigation of their role in the virus life cycle. J. Gen. Virol. 73:539-547[Abstract/Free Full Text].
20.	Melan, M. A., and G. Sluder. 1992. Redistribution and differential extraction of soluble proteins in permeabilized cultured cells. Implications for immunofluorescence microscopy. J. Cell Sci. 101:731-743[Abstract/Free Full Text].
21.	Nelle, T. D., and J. W. Wills. 1996. A large region within the Rous sarcoma virus matrix protein is dispensable for budding and infectivity. J. Virol. 70:2269-2276[Abstract/Free Full Text].
22.	Parent, L. J., R. P. Bennett, R. C. Craven, T. D. Nelle, N. K. Krishna, J. B. Bowzard, C. B. Wilson, B. A. Puffer, R. C. Montelaro, and J. W. Wills. 1995. Positionally independent and exchangeable late budding functions of the Rous sarcoma virus and human immunodeficiency virus Gag proteins. J. Virol. 69:5455-5460[Abstract/Free Full Text].
23.	Parent, L. J., C. B. Wilson, M. D. Resh, and J. W. Wills. 1996. Evidence for a second function of the MA sequence in the Rous sarcoma virus Gag protein. J. Virol. 70:1016-1026[Abstract/Free Full Text].
24.	Pearce-Pratt, R., D. Malamud, and D. M. Phillips. 1994. Role of the cytoskeleton in cell-to-cell transmission of human immunodeficiency virus. J. Virol. 68:2898-2905[Abstract/Free Full Text].
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