Rotavirus Capsid Protein VP5* Permeabilizes Membranes

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Journal of Virology, April 1999, p. 3147-3153, Vol. 73, No. 4
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Rotavirus Capsid Protein VP5* Permeabilizes Membranes

Evgeniya Denisova,¹^,² William Dowling,¹^,² Rachel LaMonica,¹^,² Robert Shaw,¹^,³ Suzanne Scarlata,⁴ Franco Ruggeri,⁵ and Erich R. Mackow¹^,²^,³^,^*

Department of Medicine,¹ Department of Molecular Genetics and Microbiology,² and Department of Physiology and Biophysics,⁴ SUNY at Stony Brook, Stony Brook, and Northport VA Medical Center, Northport,³ New York, and Instituto Superiore Di Sanita, Rome, Italy⁵

Received 29 July 1998/Accepted 29 December 1998

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Proteolytic cleavage of the VP4 outer capsid spike protein into VP8* and VP5* proteins is required for rotavirus infectivityand for rotavirus-induced membrane permeability. In this studywe addressed the function of the VP5* cleavage fragment in permeabilizingmembranes. Expressed VP5* and truncated VP5* proteins were purifiedby nickel affinity chromatography and assayed for their abilityto permeabilize large unilamellar vesicles (LUVs) preloaded withcarboxyfluorescein (CF). VP5* and VP5* truncations, but not VP4or VP8*, permeabilized LUVs as measured by fluorescence dequenchingof released CF. Similar to virus-induced CF release, VP5*-inducedCF release was concentration and temperature dependent, with apH optimum of 7.35 at 37°C, but independent of the presence ofdivalent cations or cholesterol. VP5*-induced permeability wascompletely inhibited by VP5*-specific neutralizing monoclonalantibodies (2G4, M2, or M7) which recognize conformational epitopeson VP5* but was not inhibited by VP8*-specific neutralizing antibodies.In addition, N-terminal and C-terminal VP5* truncations includingresidues 265 to 474 are capable of permeabilizing LUVs. Thesefindings demonstrate that VP5* permeabilizes membranes in theabsence of other rotavirus proteins and that membrane-permeabilizingVP5* truncations contain the putative fusion region within predictedvirion surface domains. The ability of recombinant expressed VP5*to permeabilize membranes should permit us to functionally definerequirements for VP5*-membrane interactions. These findings indicatethat VP5* is a specific membrane-permeabilizing capsid proteinwhich is likely to play a role in the cellular entry ofrotaviruses.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Rotaviruses are nonenveloped icosahedral viruses with 11 double-stranded RNA gene segments inside a 70-nm triple-layered particle(TLP) (14, 45). Four capsid proteins, VP2, VP6, VP7, and VP4,are present in infectious TLPs (14, 45). Calcium chelationremoves VP4 and VP7 outer capsid proteins and converts TLPs intotranscriptionally active but noninfectious double-layered particles(DLPs) (7, 51). Rotavirus RNAs are transcribed within DLPsby a self-contained double-stranded RNA-dependent RNA polymerasecomplex (7) and are extruded from pores in the DLP (31, 46).VP7 is the major structural protein on the surface of TLPs, whiledimeric VP4 spikes project from the rotavirus surface (14, 45,47, 53, 59). VP7 is the viral glycoprotein, while VP4 lackssignal sequences and posttranslational modifications (14). VP4and VP7 are targets of neutralizing antibodies to rotaviruses,and immune responses to these proteins protect animals from disease(14, 26, 37, 42, 43, 55).

Protease treatment of rotaviruses is required for viral infectivity. On the virion, trypsin cleaves VP4 (86 kDa) into theVP8* (28 kDa) and VP5* (60 kDa) proteins, activating the virusfor infection (13, 15). The VP4 and VP8* proteins of somerotaviruses are capable of hemagglutination through viral attachmentto sialic acid-containing cell surface components (17, 24,35). Cellular integrins are also reported to mediate interactionswith rotavirus outer capsid proteins (9). Proteolytically activatedrotaviruses enter cells rapidly by a mechanism consistent withdirect membrane penetration (25, 27, 56, 57). Cellularentry of rotaviruses occurs with a half-life of 5 min at 37°C(25, 56), and rotaviruses which are not proteolytically activatedare endocytosed and degraded but do not infect cells (25, 27,56, 57). Consistent with a direct entry mechanism, viral entryis not inhibited by lysosomotropic agents, which basify endosomes,or macrolide antibiotics, bafilomycin A, and concanamycin A, whichblock endosome acidification by selectively inhibiting the vacuolarH⁺-ATPase (11, 19, 25, 27).

Rotaviruses have also been shown to permeabilize cells, permitting ⁵¹Cr release, cell-cell fusion, ethidium bromide entry, and coentryof the cellular toxin alpha sarcin (11, 16, 25, 33, 49).TLP but not DLP rotaviruses have also been shown to permeabilizevesicles preloaded with carboxyfluorescein (CF) (40, 50).Several reports demonstrate that membrane permeability requirestrypsinization of TLPs, is temperature dependent, occurs at neutralpH, and is inhibited by monoclonal antibodies (MAbs) to outercapsid proteins VP8*, VP5*, and VP7 (11, 16, 20, 21, 25,27, 33, 40, 50). However, EGTA treatment of pretrypsinizedTLPs also reportedly permits virus to permeabilize membranes orfuse cells (16, 49). EGTA solubilizes the VP4 and VP7 outercapsid proteins of the virion (7, 51), suggesting that solubilizedouter capsid proteins are capable of permeabilizing membranesin the absence of particles or virion uncoating (16, 49).

In this report we demonstrate that the expressed VP5* protein from rhesus rotavirus (RRV) is capable of permeabilizing membranesin the absence of other rotavirus proteins or virion associations.We demonstrate that purified VP5* and truncated VP5* proteinscontaining predicted virion surface domains of VP5*, but not VP8*or VP4, permeabilize liposomes, causing the release of CF fromlarge unilamellar vesicles (LUVs). VP5*-induced CF release isdose dependent and occurs optimally at 37°C at pH 7.35. VP5*-mediatedmembrane permeabilization is blocked by MAbs which recognize aconformationally determined epitope on the VP5* protein and neutralizeRRV infectivity. Further, VP5* truncations which permeabilizeLUVs contain the putative fusion domain of VP5* (36) but donot require the new N terminus of VP5* or downstream alpha-helicalheptad repeats (residues 494 to 557) for membrane permeabilization.These findings functionally demonstrate the ability of the rotavirusVP5* protein to permeabilize membranes and suggest a requiredrole for the VP5* cleavage product in cellular permeability duringrotavirusentry.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents. Egg yolk phosphatidylcholine (PC) (L- $alpha$ -lecithin; molecular weight, 760), palmitoyl-oleoyl phosphatidylcholine (POPC), phosphatidylethanolamine (PE), and phosphatidyl serine (PS) in chloroformwere obtained from Avanti Polar Lipids, Inc. (Alabaster, Ala.).The fluorescent dye CF (molecular weight, 376) was obtained fromMolecular Probes (Eugene, Oreg.), and cholesterol was from Sigma(St. Louis, Mo.). Isopropyl- $beta$ -D-thiogalactopyranoside (IPTG) wasobtained from Lab Scientific Inc. (Livingston, N.J.). NeutralizingMAbs (N-MAbs) M2, M7, 2G4, and 7A12 have been previously described(36, 38, 55). N-MAbs M2, M7, and 2G4 require VP4 residues248 to 474, within VP5*, for recognition, while N-MAb 7A12 recognizespolypeptides containing residues 55 to 222 of VP8* (38). N-MAbshave previously been demonstrated to select neutralization escapemutants with mutations in their VP4 proteins at position 188 (MAb7A12), 388 (MAb M2), or 393 (MAbs M7 and 2G4) (36).

Cells and virus. RRV was cultivated in MA104 cells as previously described (54). MA104 cells were grown in Dulbecco modified Eagle medium(Gibco/BRL) in the presence of 10% fetal calf serum. Cells wereinfected at 0.1 focus-forming unit (FFU)/cell in serum-free medium,and medium was supplemented with trypsin (0.2 µg/ml). Infectedcells were disrupted by freezing and thawing three times followedby Genetron extraction and purification on CsCl gradients as previouslydescribed (54). TLPs at 1.36 g of CsCl per ml were collected,trypsin (2 µg/ml) activated at 37°C for 15 min, and used in thesestudies. Virus was quantitated by the Bio-Rad protein assay, andtiters of infectious virus were determined by a focus assay aspreviously described (55).

Plasmids. Specific primers for the 5' and 3' ends of the coding sequence of RRV were synthesized, with each 5'-end primer having a BamHIsite and each 3' primer having either an SstI or an XhoI site.Products containing VP4 (amino acids [aa] 1 to 776), VP8* (aa1 to 231), VP5* (aa 248 to 776), VP5*(248 to 475), and VP5*(265to 475) were generated by PCR and ligated into pET-6HIS plasmidsby standard methods. The pET-6HIS vector is a modified versionof pET30a (Novagen) containing a replacement of the NdeI-to-BamHIfragment with a methionine and six histidines in frame 1 withthe BamHI site. Ligation products were transformed into Escherichiacoli XL-1 Blue (Stratagene) and selected on kanamycin plates.Constructs were verified by restriction enzyme digestion, sequencingas previously described (36), and protein expression (seebelow).

Protein expression and purification. pET-6HIS plasmids encoding VP4, VP8*, VP5*, VP5*(248-474), or VP5*(265-474) were transformed into BL21(DE3) cells (Novagen).Single colonies were picked and grown overnight at 37°C in L brothwith 50 µg of kanamycin per ml. Overnight cultures were diluted1:20 in L broth-kanamycin, incubated at 37°C until the opticaldensity at 600 nm was 0.6, and induced with IPTG for 3 h. Cellswere harvested by centrifugation at 3,000 × g for 15 min and sonicatedin 10 mM Tris (pH 8.0)-0.1 M NaH₂PO₄-2 M urea. Supernatants werediscarded, and pellets were solubilized in 10 mM Tris (pH 8.0)-0.1M NaH₂PO₄-8 M urea (buffer B). Lysates were pelleted in a microcentrifugefor 10 min, and nickel-nitrilotriacetic acid (NTA)-agarose (Qiagen)was added to supernatants and left for 30 minutes at room temperature.NTA resin was pelleted and washed five times with buffer B containing50 mM imidazole and one time with buffer B (pH 6.3). Proteinswere eluted in buffer B containing 100 mM EDTA. Eluted proteinswere dialyzed sequentially in HEPES-buffered saline (HBS) (50mM HEPES [pH 8.0], 150 mM NaCl) containing 8, 6, 4, 2, 1, or 0.5M urea (>4 h each) and finally againstHBS.

VP5* radiolabeling and recognition. A 50-ml culture of BL21(DE3) cells containing VP5* pET-6HIS was grown to an optical density at 600 nm of 0.6 to 0.8 at 37°C.The cells were harvested by centrifugation at 3,000 × g for 15min, washed with phosphate-buffered saline, and radiolabeled (100µCi of Tran³⁵S-label per ml) in methionine- and cysteine-free Grace's medium(GIBCO) following induction with 1 mM IPTG at 37°C. Radiolabeledexpressed proteins were purified as described above on NTA resin(Qiagen). Radiolabeled VP5* was immunoprecipitated as previouslydescribed (38) with VP5*-specific (2G4) or VP8*-specific (7A12)N-MAbs (55) in radioimmunoprecipitation assay buffer containing0.1% sodium dodecyl sulfate (SDS). Proteins were analyzed by SDS-polyacrylamidegel electrophoresis (SDS-PAGE) (10% polyacrylamide), and proteinbands were visualized by fluorography. VP8* and VP4 proteins wererecognized by MAb 7A12, and VP4 was recognized by 2G4, by enzyme-linkedimmunosorbent assay as previously described (55).

Preparation of liposomes. Liposomes of PC containing CF were prepared by an extrusion method (3, 40). Briefly, 2 mg of PC was dissolved in chloroform,dried under nitrogen, and further dried under vacuum. Lipids wereresuspended in 20 µl of CF (70 mM in 10 mM Tris, pH 7.35) by vortexing.Following five cycles of freezing and thawing, LUVs were preparedby extrusion through a 0.1-µm-pore-size membrane (Mini-extruder;Avanti Polar Lipids). Extravesicular fluorophore was eliminatedby size exclusion chromatography on Sephadex G-50 (Pharmacia)in 10 mM Tris-HCl (pH 7.35)-140 mM NaCl (TN buffer) (3, 40).Fractions (150 µl) were collected, and 3 µl was assayed in 1.6ml of TN buffer for fluorescence dequenching following additionof 0.125% Triton X-100. Fluorescence dequenching was monitoredin a Perkin-Elmer LS-5B luminescence spectrometer at 520 nm (490nm for excitation) (22a). Fractions with a fluorescence changeratio of >15 were pooled and used in CF releaseassays.

CF release assays. The ability of RRV and purified RRV proteins to permeabilize LUVs and cause CF release was assayed by measuring the fluorescencedequenching of the released fluor, essentially as previously described(40, 50). CF-containing LUVs (5 to 10 µl) were equilibratedin 1.6 ml of TN buffer in fluorimeter cuvettes at 37°C for 3 minwith constant stirring prior to addition of rotavirus (10⁷ to 10⁸ FFU) or rotavirus proteins (0.1 to 25 µg). CF release was monitoredover time under various conditions as described in the figurelegends. All experiments were repeated several times with differentpreparations of liposomes, proteins, and virus. At the conclusionof each experiment, LUVs were lysed with 0.1% Triton X-100 todetermine the maximum dequenching within each sample (40). Sampleswith no added proteins or virus were incubated and similarly treatedto control for spontaneous CF release fromliposomes.

Results are expressed as percentages of total fluorescence dequenching resulting from Triton X-100 addition. The percent fluorophoredequenching was calculated according to the formula percent release= (F_t $-$ F₀)/(F_T $-$ F₀)] × 100, where F₀ is the background fluorescence,F_t is the fluorescence at time t, and F_T is the total fluorescenceof the sample (40).

The ability of VP5 to permeabilize liposomes was determined in 32 separate experiments, using freshly prepared CF-loaded liposomesand at least 21 different preparations of VP5. In order to verifythat CF was specifically released by VP5, each lot of VP5 wastested for the ability of MAb 2G4 to block its activity. No lotsof VP5 caused CF release that was not blocked by prior additionof MAb 2G4. Results from replicate samples assayed during thecourse of these experiments never varied by more than 5%.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Protein expression and purification. VP5*, VP8*, and VP4 were expressed in pET-6HIS plasmids fused to an upstream methionine and six histidine residues. FollowingIPTG induction, VP5* protein was expressed at high levels in BL21(DE3)bacteria (Fig. 1A). The N-terminal six-histidine tag conferredprotein binding to nickel, and induced proteins were purifiedon a nickel-NTA-agarose resin (Fig. 1A). Purified VP5* was eluted,dialyzed into HBS, and tested for its recognition by VP5*-specificN-MAbs 2G4, M2, and M7 (36, 55). All three N-MAbs immunoprecipitatedVP5* (results for 2G4 are shown Fig. 1C), while the VP8*-specificN-MAb, 7A12, failed to recognize VP5*. VP5* truncations containingresidues 248 to 474 or 265 to 474 were similarly expressed andpurified from pET-6HIS plasmids (Fig. 1B). Both truncated proteinsare recognized by MAbs 2G4, M2, and M7 (not shown). Since MAbs2G4, M2, and M7 recognize a conformational epitope of VP5* presenton RRV (38, 55), this indicates that purified expressed VP5*proteins are present in a conformation similar to that of thevirion outer capsid.

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FIG. 1. Expression and purification of proteins VP5*, VP4, and VP8* (A) and VP5*(248-474) and VP5*(265-474) (B) were expressed in BL21(DE3) from pET-6HIS plasmids. Bacteria were induced with IPTG (1 mM) and grown for 3 h prior to pelleting and sonication. Proteins were purified on Ni-NTA-agarose (Qiagen), and crude or purified samples were analyzed by SDS-PAGE (10% polyacrylamide for panel A and 12% polyacrylamide for panel B) and stained with Coomassie blue. (A) Lanes: 1, molecular mass standards; 2, VP5; 3, VP4; 4, VP8. (B) Lanes: 1, molecular mass standards; 2, VP5*(248-474); 3, VP5*(265-474). (C) VP5* was radiolabeled following IPTG induction of pET-6HIS VP5* plasmids in BL21(DE3) with 100 µCi of Tran³⁵S-label per ml in methionine- and cysteine-free Grace's medium. VP5* was purified on Ni-NTA-agarose as described above. VP5* was analyzed directly by SDS-PAGE (10% polyacrylamide) (lane 1) or immunoprecipitated with MAb 264 (lane 3), MAb 7A12 (lane 4), or normal mouse serum (lane 5). Lane 2, molecular mass standards. Proteins were visualized by fluorography.

VP5* permeabilize LUVs. Trypsinized rotavirus TLPs as well as outer capsid proteins released from the virion by calcium chelation are capable of permeabilizingmembranes (40, 49, 50). In these experiments the abilityof the purified expressed VP5* protein to permeabilize membraneswas tested by using LUVs preloaded with CF. Fluorescence dequenchingand an increase in fluorescence at 520 nm result from permeabilizationof CF-loaded LUVs (40). Similar to the case for trypsinizedTLPs, addition of purified VP5* protein to LUVs resulted in 80to 90% CF release in 30 min at 37°C (Fig. 2). In contrast, LUVsalone or the addition of VP8* or VP4 proteins did not cause CFrelease from LUVs (Fig. 2). Triton X-100 addition at the conclusionof experiments completely released CF from LUVs, demonstratingthat the assay mixtures contained equivalent amounts of CF-loadedLUVs.

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FIG. 2. VP5* permeabilizes LUVs. Purified LUVs containing CF (70 mM) were incubated in 1.6 ml of TN buffer at 37°C with or without prior addition of 100 µl of trypsin-activated RRV (0.5 mg/ml; 10⁹ FFU/ml) or nickel affinity-purified VP4 (5 µg; 37.5 nM), VP8* (10 µg; 240 nM), or VP5* (4 µg; 44 nM). VP4 and VP8* failed to induce CF release over the entire range of protein concentrations tested (VP8*, 5 to 25 µg [120 to 600 nM]); VP4, 1 to 10 µg [7.5 to 75 nM]). Fluorescence dequenching of samples was monitored at various times at 520 nm in an LS-5B luminescence spectrometer following excitation at 490 nm. After 30 min, Triton X-100 (0.125%) was added in order to assess the total CF content of each sample, which was quantitated as described in Materials and Methods. This experiment was repeated three times with similar results.

Neutralizing MAbs to VP5* completely inhibit CF release. VP5*-specific MAbs were used to demonstrate that LUVs were specifically permeabilized by the VP5* protein. VP5*-specific antibodiesM2, 2G4, and M7 neutralize RRV infectivity through the recognitionof a conformationally determined epitope on the virion surface(38, 55). VP5*-specific N-MAbs (2G4, M2, and M7) or a VP8*-specificN-MAb (7A12) (1 µl of ascites fluid) was incubated with VP5* for30 min at room temperature prior to the addition of VP5* to LUVs.RRV was incubated with MAb 2G4 for 15 min prior to addition toCF-containing liposomes as previously described (50). Additionof the VP8*-specific MAb, 7A12, to VP5* had no effect on VP5*-inducedCF release (Fig. 3). In contrast, addition of VP5*-specific N-MAbscompletely blocked the ability of VP5* to permeabilize LUVs. Theability of 2G4 to inhibit rotavirus-mediated CF release in thisexperiment corresponds to the results of Ruiz et al. (50). Thesefindings demonstrate the specificity of VP5*-induced membranepermeabilization in the CF release assay and further indicatethat VP5*-specific N-MAbs block the ability of VP5* to permeabilizemembranes.

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FIG. 3. VP5*-specific N-MAbs block VP5*-induced membrane permeability. VP5*-specific (2G4, M2, and M7) or VP8*-specific (7A12) MAbs were incubated with purified VP5* (4 µg; 44 nM) or 100 µl of trypsin-activated RRV (0.5 mg/ml; 10⁹ FFU/ml) at room temperature for 30 min prior to addition to CF-loaded LUVs in 1.6 ml of TN buffer at 37°C. At various time points, fluorescence dequenching of samples was monitored in a fluorimeter at an excitation wavelength of 490 nm and an emission wavelength of 520 nm. After 30 min, Triton X-100 (0.125%) was added in order to assess the total CF content of each sample, which was quantitated as described in Materials and Methods. This experiment was repeated two times with similar results. The specific function of each lot of VP5 was tested with MAb 2G4 in a CF release assay (see Materials and Methods).

Determinants of VP5*-induced membrane permeability. The requirements for VP5*-induced membrane permeability were tested under a number of conditions. Addition of increasing amountsof VP5* to membranes demonstrated that VP5*-induced CF releaseis concentration dependent (Fig. 4A). Equilibration of liposomesin buffers of various pHs or temperatures further demonstratedthat VP5*-induced membrane permeability is optimal at neutralpH (pH 7.35) at 37°C (Fig. 4B and C).

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FIG. 4. Conditions of VP5*-induced membrane permeability. VP5* was added to CF-loaded LUVs under various conditions. (A) Increasing amounts of purified VP5* (1 µg [11 nM], 2 µg [22 nM], 4 µg [44 nM], or 6 µg [66 nM]) were added to LUVs. This experiment was repeated two times with similar results. (B) VP5* (4 µg; 44 nM) was incubated with LUVs in TN buffer at various pHs, and results were corrected for spontaneous CF release at identical pHs. This experiment was repeated six times with similar results. (C) VP5* (4 µg; 44 nM) and LUVs were incubated as described above at 4, 22, 37, or 43°C. This experiment was repeated five times with similar results. (D) Egg yolk PC or PC-cholesterol (10:1) LUVs were preloaded with CF and purified by Sephadex G-50 chromatography. This experiment was repeated three times with similar results. The ability of the VP5* (4 µg; 44 nM) to permeabilize PC liposomes with or without the inclusion of cholesterol was monitored over time. Fluorescence dequenching of samples was monitored in a fluorimeter at an excitation wavelength of 490 nm and an emission wavelength of 520 nm. After 22 min (B), 27 min (D), or 30 min (A and C), the total CF content of each sample was assessed by addition of Triton X-100 (0.125%) and quantitated as described in Materials and Methods.

Rotaviruses are sensitive to calcium concentration and are converted from infectious TLPs to noninfectious but transcriptionallyactive DLPs by reduced intracellular [Ca²⁺] (7, 51). However, the addition of 5 mM CaCl₂, MgCl₂, MnCl₂,or ZnCl₂ to CF-containing LUVs had no effect on VP5*-induced CFrelease (not shown). VP5* also permeabilized LUVs with variouslipid compositions, including POPC, PS, or PE at a 1:1 ratio withPC (not shown). Additionally there was no detectable differencein VP5*-induced CF release from PC or POPC CF-loaded LUVs. Cholesterolhas also been suggested to be a requirement for rotavirus-mediatedmembrane permeability (16, 21). Figure 4D demonstrates theability of the VP5* protein to permeabilize PC liposomes withor without the inclusion of cholesterol (PC/cholesterol ratio,10:1).

VP5* truncations permeabilize LUVs. Single amino acid changes within the VP5* protein at residues 388 and 393 are selected by N-MAbs M2, M7, and 2G4 within theputative fusion domain of VP5* (36). Further mapping of theseantibodies by deletional analysis defined that the VP5*(248-474)fragment (residues 248 to 474) was required for recognition bythe VP5*-specific N-MAbs (38). Additionally, cleavage of VP4following residue 247 has recently been shown to be required forvirus-like particle (VLP)-mediated membrane permeabilization (20).In order to determine whether the N terminus of VP5* is requiredfor VP5* function and whether VP5*(248-474) MAb recognition domainsare sufficient for VP5*-induced membrane permeabilization, weinvestigated the ability of truncated VP5* proteins to permeabilizeLUVs. Similar to VP5*, both VP5*(248-474) and VP5*(265-474) werecapable of permeabilizing LUVs (Fig. 5). Further, the abilityof the VP5* truncation proteins to permeabilize membranes wascompletely inhibited by prior incubation with VP5*-specific N-MAb2G4 (Fig. 5). This demonstrates that VP5* truncations containingpredicted extravirion domains of VP5* are functional in membranepermeabilization and that a VP5* truncation containing residues265 to 474 is recognized by N-MAb 2G4. Additionally, N-terminalresidues of VP5*, resulting from trypsin cleavage of VP4 afterresidue 247 on the virion, are not required for purified VP5*to permeabilize membranes.

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FIG. 5. VP5* truncations permeabilize LUVs. Purified LUVs containing CF were incubated in 1.6 ml of TN buffer at 37°C for 30 min with purified VP5* (6 µg; 67 nM) or truncation VP5*(248-474) (3 µg; 72 nM) or VP5*(265-474) (3 µg; 78 nM). As for Fig. 3, aliquots were also incubated with VP5*-specific N-MAb 2G4 at room temperature for 30 min prior to incubation with LUVs. Fluorescence dequenching of samples was monitored in a fluorimeter at an excitation wavelength of 490 nm and an emission wavelength of 520 nm. After 22 min, the total CF content of each sample was assessed by addition of Triton X-100 (0.125%) and quantitated as described in Materials and Methods. This experiment was repeated three times with similar results.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Although fusion proteins which mediate the entry of enveloped viruses have been extensively investigated, the ability of nonenvelopedviruses to cross cellular membranes and enter cells is poorlyunderstood. In this study we have demonstrated that the purifiedrotavirus VP5* protein is capable of permeabilizing membranesin the absence of other rotavirus proteins. Like virus-inducedmembrane permeability, VP5*-induced membrane permeability is optimalat 37°C at neutral pH (40). VP5* truncations containing predictedextravirion domains are similarly active in permeabilizing membranes.These findings implicate the outer capsid protein VP5* in permeabilizingmembranes during rotavirus entry and further suggest that trypsincleavage of VP4 may be required to effect conformational changesin VP5* which permit VP5*-membraneinteractions.

VP5*-mediated membrane permeabilization is blocked by N-MAbs which recognize a conformationally determined epitope of VP5*on the virion (38, 55). This demonstrates that apparentlynative VP5* is functional in permeabilizing membranes and furthersuggests that VP5*-specific N-MAbs may neutralize rotavirus bypreventing virus-membrane interactions and cellular entry. Neutralizingantibodies to VP7 or VP8* have also been demonstrated to inhibitTLP-induced membrane permeability (11, 16, 33, 50). However,the function of VP5* in permeabilizing membranes suggests thatantibodies to VP8* and VP7 may block membrane permeability indirectly,perhaps by altering conformational changes in VP5*, by stericallyinhibiting VP5*-membrane interactions, or by preventing cell attachmentor virion uncoating. However, our studies do not exclude the possibilitythat VP8* or VP7 has membrane-permeabilizing functions, and arole for VP7 in permeabilizing membranes has been suggested (4).In these studies there was no evidence that VP8* or uncleavedVP4 was capable of permeabilizingmembranes.

Antibodies to VP5* were previously used to generate neutralization escape mutants with single amino acid changes within theVP5* protein selected by N-MAbs M2 M7 and 2G4 at residues 388and 393 (36). Further mapping of these antibodies by deletionalanalysis defined the VP5*(248-474) fragment (residues 248 to 474)required for recognition by the VP5*-specific N-MAbs (38). Twotruncated VP5* proteins were functionally analyzed in these experiments,the VP5*(248-474) fragment and a short N-terminal truncation ofVP5*(265-474). Both VP5 truncations were capable of permeabilizingmembranes, but permeabilization was completely blocked by preincubatingtruncations with N-MAb2G4.

We previously reported that VP5 contains a hydrophobic putative internal "fusion" domain (VP5 HD) (residues 385 to 404) whichhas homology with the fusion domains of the E1 proteins of Sindbisvirus and Semliki Forest virus (36). Interestingly, the identicalGGA sequence required for the function of the Semliki Forest virusE1 fusion peptide (residues 90 to 92) is present in the VP5* HDand conserved in all rotaviruses (28, 29, 30, 32, 36).An additional diglycine motif flanks the VP5* HD, and five helix-breakingglycine and proline residues, which are highly conserved amongrotaviruses, confer a random coiled structure to the VP5* HD.Glycine residues have recently been identified as key elementsin vesicular stomatitis virus G protein-induced membrane fusion(6).

Although rotaviruses do not normally fuse cells, studies using a rotavirus cell-cell fusion assay showed a requirement forcholesterol for rotavirus-induced cell fusion (16, 20, 21).Cholesterol is not required for rotavirus permeabilization ofmodel membranes (40, 50), and from our studies, VP5* proteinscontaining VP5* HD mediate membrane permeabilization which ischolesterol independent. As a result, cholesterol may be a specificrequirement of the cell-cell fusion assay but not a specific requirementof VP5*-induced membranepermeabilization.

Recently, VLPs with mutagenized VP4 trypsin cleavage sites were used to demonstrate that cleavage following residue 247 wasrequired for VLP-induced cell-cell fusion (20). The specificitysuggested that the new amino terminus of VP5* was required formembrane permeabilization and that additional residues presenton VP5* might block VP5* membrane functions. However, in thisstudy each of the expressed VP5* proteins contains an additionalmethionine and six histidine residues added to the N terminusof VP5*, and the addition of these residues does not block VP5*-mediatedmembrane permeabilization. In addition, the VP5*(265-474) truncation,with the N-terminal 17 residues of VP5* deleted, is functionalin membrane permeabilization. These results suggest that specificVP4 cleavage is a requirement for the function of VP5* on thevirion and is not a functional requirement of the VP5*polypeptide.

Other nonenveloped viruses, like poliovirus, reovirus, and adenovirus, have been suggested to mediate interactions with membranesduring viral entry (2, 5, 8, 12, 18, 22, 23,39, 41, 48, 52, 58). However, specific proteins fromthese viruses have not been demonstrated to have membrane-permeabilizingactivity. The ability of the rotavirus VP5* protein to permeabilizemembranes suggests that additional nonenveloped viruses are likelyto have specific proteins which effect membrane permeability duringviralentry.

Hypotheses for how rotavirus outer capsid proteins permeabilize membranes have also been suggested (16, 33, 49, 50).Reduced intracellular calcium levels within early endosomes havebeen suggested to uncoat rotavirus outer capsid proteins, whichthen permeabilize and lyse the early endosome, effecting viralentry (49). It has also been suggested that outer capsid proteinson the virion first permeabilize cellular membranes, permittingcalcium efflux from the early endosome (49). The reduced-calciumenvironment causes subsequent conformational changes, and outercapsid uncoating disrupts the early endosomal membrane attachedto the virion (49). It is also possible that a focal permeabilizationof the cellular membrane occurs and permits a localized calciumflux in the virion which effects virion uncoating and membranedisruption.

The ability of VP5* to permeabilize membranes is consistent with all of these possibilities. However, it has yet to be determinedwhether VP5* lyses or selectively permeabilizes membranes. Thedelivery of rotavirus 50-nm particles into cells is relativelycomplex, involving both membrane permeability and conformationalchanges in the virion which could contribute to particle entryand membrane disruption. In contrast, the use of purified VP5*in studies of membrane permeability should permit us to defineVP5* functions in membrane interactions and discern the role ofVP5* in the rotavirus entry process. Additionally, the abilityto selectively mutagenize VP5* should further define the domainsand residues of VP5* which are required for membrane binding andpermeability.

	ACKNOWLEDGMENTS

We are grateful to Erwin London and Irina Gavrilovskaya for insightful discussions of these studies. We thank Mary Ellen Fayand Yildiz Farooqui for technicalassistance.

This work was supported by a Merit Award from the Veterans Administration and by NIH grants R01-AI31016 and RO3-AI42150 toE.R.M.

	FOOTNOTES

^* Corresponding author. Mailing address: Departments of Medicine and Microbiology, HSC T17, Rm. 60, SUNY at Stony Brook, StonyBrook, NY 11794-8173. Phone: (516) 444-2120. Fax: (516) 444-8886.E-mail: EMackow{at}mail.som.sunysb.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Arias, C. F., P. Romero, V. Alvarez, and S. Lopez. 1996. Trypsin activation pathway of rotavirus infectivity. J. Virol. 70:5832-5839[Abstract].
2.	Blumenthal, R., P. Seth, M. C. Willingham, and I. Pastan. 1986. pH-dependent lysis of liposomes by adenovirus. Biochemistry 25:2231-2237[Medline].
3.	Butko, P., F. Huang, M. Pusztai-Carey, and W. K. Surewicz. 1996. Membrane permeabilization induced by cytolytic delta-endotoxin CytA from Bacillus thuringiensis var. israelensis. Biochemistry 35:11355-11360[Medline].
4.	Charpilienne, A., M. J. Abad, F. Michelangeli, F. Alvarado, M. Vasseur, J. Cohen, and M. C. Ruiz. 1997. Solubilized and cleaved VP7, the outer glycoprotein of rotavirus, induces permeabilization of cell membrane vesicles. J. Gen. Virol. 78:1367-1371[Abstract].
5.	Chow, M., J. F. Newman, D. Filman, J. M. Hogle, D. J. Rowlands, and F. Brown. 1987. Myristylation of picornavirus capsid protein VP4 and its structural significance. Nature 327:482-486[Medline].
6.	Cleverley, D. Z., and J. Lenard. 1998. The transmembrane domain in viral fusion: essential role for a conserved glycine residue in vesicular stomatitis virus G protein. Proc. Natl. Acad. Sci. USA 95:3425-3430[Abstract/Free Full Text].
7.	Cohen, J., J. Laporte, A. Charpilienne, and R. Scherrer. 1979. Activation of rotavirus RNA polymerase by calcium chelation. Arch. Virol. 60:177-186[Medline].
8.	Cotten, M., M. Saltik, M. Kursa, E. Wagner, G. Maass, and M. L. Birnstiel. 1994. Psoralen treatment of adenovirus particles eliminates virus replication and transcription while maintaining the endosomolytic activity of the virus capsid. Virology 205:254-261[Medline].
9.	Coulson, B. S., S. L. Londrigan, and D. J. Lee. 1997. Rotavirus contains integrin ligand sequences and a disintegrin-like domain that are implicated in virus entry into cells. Proc. Natl. Acad. Sci. USA 94:5389-5394[Abstract/Free Full Text].
10.	Crawford, S. E., M. Labbe, J. Cohen, M. H. Burroughs, Y. J. Zhou, and M. K. Estes. 1994. Characterization of virus-like particles produced by the expression of rotavirus capsid proteins in insect cells. J. Virol. 68:5945-5922[Abstract/Free Full Text].
11.	Cuadras, M. A., C. F. Arias, and S. Lopez. 1997. Rotaviruses induce an early membrane permeabilization of MA104 cells and do not require a low intracellular Ca²⁺ concentration to initiate their replication cycle. J. Virol. 71:9065-9074[Abstract].
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