Optimal Replication Activity of Vesicular Stomatitis Virus RNA Polymerase Requires Phosphorylation of a Residue(s) at Carboxy-Terminal Domain II of Its Accessory Subunit, Phosphoprotein P

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Journal of Virology, July 1999, p. 5613-5620, Vol. 73, No. 7
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Optimal Replication Activity of Vesicular Stomatitis Virus RNA Polymerase Requires Phosphorylation of a Residue(s) at Carboxy-Terminal Domain II of Its Accessory Subunit, Phosphoprotein P

Leroy N. Hwang,¹ Nathan Englund,¹ Tapas Das,² Amiya K. Banerjee,² and Asit K. Pattnaik¹^,^*

Department of Microbiology and Immunology, University of Miami School of Medicine, Miami, Florida 33136,¹ and Department of Virology, The Cleveland Clinic Foundation, Cleveland, Ohio 44195²

Received 3 September 1998/Accepted 29 March 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The phosphoprotein, P, of vesicular stomatitis virus (VSV) is a key subunit of the viral RNA-dependent RNA polymerase complex.The protein is phosphorylated at multiple sites in two differentdomains. We recently showed that specific serine and threonineresidues within the amino-terminal acidic domain I of P proteinmust be phosphorylated for in vivo transcription activity, butnot for replication activity, of the polymerase complex. To examinethe role of phosphorylation of the carboxy-terminal domain IIresidues of the P protein in transcription and replication, wehave used a panel of mutant P proteins in which the phosphateacceptor sites (Ser-226, Ser-227, and Ser-233) were altered toalanines either individually or in various combinations. Analysesof the mutant proteins for their ability to support replicationof a VSV minigenomic RNA suggest that phosphorylation of eitherSer-226 or Ser-227 is necessary for optimal replication activityof the protein. The mutant protein (P_226/227) in which both ofthese residues were altered to alanines was only about 8% activein replication compared to the wild-type (wt) protein. Substitutionof alanine for Ser-233 did not have any adverse effect on replicationactivity of the protein. In contrast, all the mutant proteinsshowed activities similar to that of the wt protein in transcription.These results indicate that phosphorylation of the carboxy-terminaldomain II residues of P protein are required for optimal replicationactivity but not for transcription activity. Furthermore, substitutionof glutamic acid residues for Ser-226 and Ser-227 resulted ina protein that was only 14% active in replication but almost fullyactive in transcription. Taken together, these results, alongwith our earlier studies, suggest that phosphorylation of residuesat two different domains in the P protein regulates its activityin transcription and replication of the VSVgenome.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The RNA-dependent RNA polymerase of the prototypic rhabdovirus, vesicular stomatitis virus (VSV), is comprised of two virallyencoded proteins: the large protein, L, and the phosphoprotein,P (1, 18, 20). A complex containing both the L and P proteinscarries out transcription and replication of the viral genome(see reference 1 for a review). The template recognized bythe RNA polymerase complex is the viral nucleocapsid, which containsthe ~11-kb-long negative-sense genomic RNA surrounded by the viralRNA-binding nucleocapsid protein, N. During transcription, thenucleocapsid template is utilized by the RNA polymerase complexto generate subgenomic, capped, and polyadenylated mRNAs, whichare translated to produce the viral proteins. During replication,the same RNA polymerase is believed to be switched from transcriptiveto replicative mode to synthesize a full-length, positive-sensecomplementary RNA (or antigenomic RNA) encapsidated by the N protein,which serves as the template for synthesis of progenynucleocapsids.

Biochemical and mutational studies have suggested that the L protein is multifunctional and carries the catalytic center forpolymerization of ribonucleotides during RNA synthesis (50,51). It presumably also carries other enzymatic activities,including methyltransferase, guanylyltransferase, and poly(A)polymeraseactivities necessary for generation of mature viral mRNAs (27-29,32). The multifunctional P protein, on the other hand, is requiredfor the manifestation of the functions of the L protein (1)and plays key roles in both transcription and replication of theviral genome. It interacts specifically with the L protein toform the polymerase complex of the virion (21) as well as stabilizingthe L protein against proteolytic degradation (9). It interactswith the terminal sequences of the viral genome (33, 34),presumably for viral RNA synthesis. The P protein also interactswith the N protein to form soluble N-P complexes required forencapsidation of nascent RNA chains during replication (36,48). Furthermore, P interacts with itself to form oligomersthat are required for transcription (15, 23, 24).

The P proteins of both the Indiana (P_I) and New Jersey (P_NJ) serotypes of VSV are highly acidic and consist of 265 and 274amino acids, respectively. Although these two proteins have only30% similarity at the primary sequence level, three functionallyhomologous domains (Fig. 1A) have been defined in mutational studies(25, 47). Domain I, spanning residues from 1 to about 150,is the amino-terminal acidic domain and is phosphorylated. DomainII spans from residues 210 to about 244 and is also phosphorylated.Domain III consists of 21 to 25 residues at the extreme carboxyterminus of the protein and is highly basic. Between domains Iand II, a hypervariable region (called the hinge) of approximately50 to 60 amino acids is present, but its function is unknown.

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FIG. 1. (A) Domain structure of the P protein of VSV (Indiana serotype). The P protein with the three functionally defined domains (I, II, and III) and the hinge region is shown. The phosphate acceptor sites (Ser-226, Ser-227, and Ser-233) within domain II are represented by solid circles. (B) Various mutant P proteins with substitutions of alanine (A) or glutamic acid (E) residues in place of serine residues are shown.

In the virion core as well as in infected cells, different phosphorylated forms of the P protein have been shown to exist(6, 13, 30, 31). Furthermore, functional P proteins withdifferent degrees of phosphorylation have been documented (10,35, 41, 49). It has been shown that the unphosphorylatedform of P protein is inactive in transcription in vitro (2,3). However, it becomes transcriptionally active when firstphosphorylated by cellular casein kinase II (CKII) (3, 4,15). The acceptor sites for CKII-mediated phosphorylation havebeen mapped to Ser-60, Thr-62, and Ser-64 in domain I of P_I (12,52) and Ser-59 and Ser-61 of P_NJ (53). Phosphorylation ofthese residues was recently shown to mediate the multimerizationof P protein that facilitates complex formation with the L protein(15, 23, 24). Using a panel of mutant P_I proteins in whichthe phosphorylation sites in domain I were altered to alanines,we recently showed that phosphorylation of these domain I residuesis necessary for the function of the P protein in transcriptionin vivo (45). The replication functions of the P protein invivo were unaffected by the phosphorylation status of the domainI residues. Based on these studies, it was proposed that an increasein net negative charge in this region of the protein as a resultof phosphorylation is crucial for transcriptional activation ofthe P protein (45). However, in a separate study, low levels(~25%) of transcription under in vitro conditions were observedwith a phosphorylation-defective P mutant protein (52).

Phosphorylation of serine residues in domain II also seems to control the activity of the P protein in RNA synthesis. It wasshown that phosphorylation of two specific residues (Ser-236 andSer-242) in domain II of P_NJ by L-associated kinase (LAK) is necessaryfor in vitro transcription activity of the P protein (11). ForP_NJ, domain I must be phosphorylated prior to LAK-mediated phosphorylationof domain II residues (4). P_I seems to be different in thisrespect, since domain II residues can be phosphorylated by LAKwithout prior phosphorylation of domain I residues (12). However,in a separate study, it was shown that substitution of asparticacid residues at S-60 and T-62 in domain I of P_I results in aprotein that is not phosphorylated at other sites (24). Sincephosphorylation in domain I is necessary and sufficient for transcription,it appears that phosphorylation of domain II residues may notbe involved in transcription (23, 40). In P_I, the Ser-226and Ser-233 residues are homologous to Ser-236 and Ser-242 residuesin P_NJ and were therefore proposed to be the potential sites ofphosphorylation (23). However, the actual sites of phosphorylationhave recently been mapped to Ser-226 and Ser-227 residues in P_I(12).

To examine the role of phosphorylation of domain II residues in the function of P protein in VSV RNA transcription and replicationin vivo, we have used a panel of mutant P proteins with alaninesubstitutions at the phosphate acceptor sites. Analysis of themutant P proteins for their ability to support replication ofa VSV minigenomic template in vivo showed that phosphorylationof the serine residue at either 226 or 227 is necessary for optimalreplication activity of P protein. In vivo-transcription activitiesof the mutant P proteins were unaffected. Furthermore, substitutionof negatively charged glutamic acid residues for these serineresidues resulted in a protein that was only 14% as active asthe wild-type protein in replication while retaining almost fullactivity in transcription. These results suggest that phosphorylationof domain II residues is required for optimal replication, butnot for transcription, function of the Pprotein.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and viruses. Growth and maintenance of baby hamster kidney (BHK-21) cells (ATCC CCL10) have been described previously (46). VSV (Indianaserotype; San Juan strain) was grown, and infectivity titers weredetermined in BHK-21 cells. The recombinant vaccinia virus (vTF7-3)containing the bacteriophage T7 RNA polymerase gene (22) wasgrown in BHK-21 cells, and infectivity titers of stock vTF7-3were determined as described earlier (45).

VSV protein- and minigenome-expressing plasmids. The plasmids encoding the wild-type P protein (P_wt) or various mutant P proteins (P₂₂₆, P₂₂₇, P₂₃₃, P_226/227, P_226/233, P_227/233,and P_226/227/233) of VSV (Indiana serotype; Mudd-Summers strain)in pET-3a vector have been described previously (12). Thesemutant P proteins contain serine-to-alanine amino acid substitutionsat positions 226, 227, 233, 226-227, 226-233, 227-233, and 226-227-233,respectively, within domain II of the P protein (Fig. 1). TheP_EE mutant contains glutamic acid residues in place of serineresidues at positions 226 and 227 of wild-type P protein. PlasmidspN and pL, carrying the coding regions for VSV (Indiana serotype;San Juan strain) proteins N and L, respectively, under the controlof the T7 RNA polymerase promoter, have been reported before (46).Construction of the plasmid p9BN, encoding an antigenomic-senseVSV minigenome, has also been described earlier (39).

Virus infections and DNA transfections. The details of the virus infection and DNA transfection procedures have been described in our earlier publications (44,45). Briefly, BHK-21 cells in 60-mm-diameter plates or in 35-mm-diametersix-well plates were grown to approximately 90% confluency. Thesecells were infected with vTF7-3 at a multiplicity of infectionof 10 PFU per cell. Following virus adsorption at 37°C for 45min, the cells were washed with serum-free Dulbecco's modifiedminimal essential medium (DMEM) and transfected with various combinationsof plasmid DNAs encoding the VSV proteins and the minirepliconRNA by using Lipofectin reagent (Gibco/BRL, Gaithersburg, Md.)or a transfection reagent prepared in the laboratory as describedpreviously (8). At 4 h posttransfection, the medium was removedfrom the transfected cells and the cells were washed twice inDMEM supplemented with 2% fetal bovine serum (FBS) and incubatedat 37°C with an appropriate volume of the same medium for differentlengths of time before metabolic labeling with radioactive precursors.Unless specifically described in the figure legends, in most experiments,3 µg of pN, 2 µg of pET-3P, 1 µg of pL, and 5 µg of p9BN plasmidswere used in transfection of cells in 60-mm-diameter plates. Theseplasmid amounts were reduced by half for cells in six-wellplates.

Metabolic labeling and analysis of proteins. [³⁵S]methionine labeling of proteins in transfected cells, immunoprecipitation, and subsequent sodium dodecyl sulfate-polyacrylamidegel analysis of the proteins have been described previously (45).P proteins were immunoprecipitated by using a rabbit anti-P (Indianaserotype; Mudd-Summers strain)antibody.

Metabolic labeling and analysis of transcription and replication products. Following incubation of transfected cells for 15 to 16 h at 37°C, the cells were pretreated with 15 µg of actinomycin D perml of DMEM plus FBS at 37°C for 45 min. The cells were then labeledwith 15 µCi of [³H]uridine and/or 15 µCi of [³H]adenosine per ml of DMEM plus FBS containing actinomycin D.The labeling of RNAs was performed for 6 to 8 h at 37°C. Cytoplasmicextracts from these cells were prepared in lysis buffer as describedearlier (46). The labeled RNA replication products in nucleocapsidswere immunoprecipitated by polyclonal anti-VSV antibodies andrecovered by extraction with phenol and chloroform and precipitationwith ethanol. The recovered RNAs were then separated by electrophoresisin agarose-urea gels (38) and detected by fluorography (37)as described in detail previously (46). For transcription analysis,total RNA from the cytoplasmic extracts was purified by extractionwith phenol and chloroform and recovered by precipitation withethanol. To generate VSV mRNAs, the cells were infected with VSVat a multiplicity of infection of 10 and labeled with [³H]uridine at 2 to 6 h postinfection in the presence of actinomycinD. Total RNA was recovered from the cytoplasmic extracts. TheRNAs were analyzed by electrophoresis and fluorography as describedabove. The quantitation of replication and transcription productRNAs was carried out by densitometric scanning of the fluorogramswith an IS-1000 digital imaging system version 2.02 (Alpha InnotechCorporation, San Leandro, Calif.). The readout values from thescanner provide integrated intensities of the appropriate bandsin the fluorograms. The relative levels of replication and transcriptionsupported by various mutants were calculated, with the valuesobtained for the wild-type P protein as 100. For normalizationof levels of transcription supported by the mutant P proteins,we used the following formula: normalized levels of transcription= relative levels of transcription/relative levels of replication×100.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The phosphorylation of serine residues at positions 236 and 242 within domain II of P_NJ was shown previously to play a majorrole in the function of P protein in transcription in vitro (11).Based on amino acid sequence homology, corresponding serine residuesat positions 227 and 233 of P_I were proposed to be the potentialsites for phosphorylation (23). Recently, however, biochemicaland mutational studies identified serine residues at positions226 and 227 to be the sites of phosphorylation (12). To examinethe role of phosphorylation of these residues in P protein functionin transcription and replication, we used a series of mutant Pproteins (Fig. 1B) in which serine residues at positions 226,227, and 233 were altered to alanines either individually (inmutants P₂₂₆, P₂₂₇, and P₂₃₃) or in various combinations (in mutantsP_226/227, P_226/233, P_227/233, and P_226/227/233). In initial experiments,we found that in transfected cells, the mutant P proteins wereexpressed at levels similar to that of the wild-type P proteinand the amount of P protein expression was roughly proportionalto the amount of plasmid transfected into the cells within a rangeof 1 to 15 µg. Furthermore, in pulse-chase experiments, the mutantproteins were stable over an 8-h chase period (data notshown).

In our earlier studies, we showed that the wild-type P protein of the Mudd-Summers strain of VSV functions as well as theSan Juan strain of VSV P protein in transcription and replicationwith San Juan N and L proteins (45); therefore, the above-mentionedmutant P proteins of the Mudd-Summers strain were used in orderto test their abilities to support transcription and replicationin the presence of the N and L proteins of San JuanVSV.

Phosphorylation-defective mutant P proteins do not support optimal replication of VSV. To examine the ability of the mutant P proteins to support replication of a VSV minigenome, we used a plasmid encoding anantigenomic-sense VSV minireplicon (9BN) RNA (39). The minirepliconRNA contains the terminal sequences of the VSV antigenome flankingthe sequences of the N gene and part of the L gene (39). Incells transfected with the plasmid along with the plasmids encodingthe viral proteins N, P, and L, the antigenomic-sense minirepliconRNA is replicated and amplified to generate the genomic- and antigenomic-senseRNAs (39). However, the genomic-sense RNA replication productscan be more readily detected by metabolic labeling of the transfectedcells, since the genomic RNAs are synthesized in much greatermolar abundance than the antigenomic-sense RNAs. To perform theexperiment, BHK-21 cells infected with vTF7-3 were transfectedwith plasmids encoding the minireplicon and N, L, and the wild-typeor mutant P proteins. [³H]uridine- and [³H]adenosine-labeled RNAs synthesized in the presence of actinomycinD were recovered from immunoprecipitated nucleocapsids and analyzedby electrophoresis. The results (Fig. 2) from a typical experimentshow that the mutant P proteins P₂₂₆, P₂₂₇, P₂₃₃, P_226/233, andP_227/233 (Fig. 2, lanes 4 to 6, 8, and 9) were as active as thewild-type P protein (Fig. 2, lane 3) in replication, since theamounts of replication product obtained with the mutant proteinswere comparable to that of the wild-type P protein. However, thereplication activities of the mutant proteins P_226/227 (Fig. 2,lane 7) and P_226/227/233 (lane 10) were significantly less thanthat of the wild-type P protein. In three to five independentexperiments, the average replication activity of P_226/227 andP_226/227/233 mutants was found to be 8 and 13%, respectively (Table1; also see Fig. 5) of that of the wild-type protein.

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FIG. 2. Replication of a VSV antigenomic minireplicon with P mutants. BHK-21 cells in 60-mm-diameter plates were infected with vTF7-3 and transfected with plasmids encoding the minigenomic RNA and the N, L, and wild-type or mutant P proteins. At 16 h posttransfection, the cells were labeled with [³H]uridine and [³H]adenosine in the presence of actinomycin D for 6 h. The replicated RNAs were recovered by immunoprecipitation and analyzed by electrophoresis. The arrow indicates the negative-sense replication product. The asterisk shows the transcription product which is sometimes nonspecifically immunoprecipitated by anti-VSV antibodies. G and N at left represent the G mRNA and N mRNA of VSV isolated from infected cells labeled with [³H]uridine.

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TABLE 1. Relative levels of replication and transcription by various mutant P proteins^a

We also examined whether it is possible to rescue higher levels of replication with increasing or decreasing amounts of P_226/227in transfected cells. Initially, we determined the amounts ofthe P_wt and P_226/227 proteins synthesized in cells transfectedwith various amounts of the corresponding plasmids. We found thatthe wild-type and mutant proteins were synthesized in equivalentamounts, and a linear relationship was found to exist betweenthe amounts of the expressed proteins and the amounts of the correspondingplasmid DNA used in transfection (Fig. 3A and 3B). When the levelsof replication with various amounts of P_226/227 were examined,it was found that the levels of replication increased as the amountof P_226/227 plasmid was increased and reached a maximum with 2µg of the plasmid (Fig. 3C, lane 4). However, this level representedonly 8% of that obtained with 2 µg of the plasmid encoding thewild-type protein (Fig. 2 and Table 1). The results (Fig. 3C)indicated that higher levels of replication could not be rescuedwith altered amounts of P_226/227 protein. These results suggestthat substitution of alanine for serine residues at 226 and 227renders the protein significantly less active in replication andthat serine residue at position 233 may not have a role in thereplication activity of the protein. Since the serine residuesat both 226 and 227 have been shown to be phosphorylated (12),the results further suggest that phosphorylation of the serineresidue at either 226 or 227 is sufficient to achieve optimalreplication activity of the protein.

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FIG. 3. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysis of immunoprecipitated wild-type (A) and P_226/227 (B) proteins expressed in cells transfected with various amounts (indicated in micrograms above each lane) of the plasmids. The expressed proteins are shown by the arrows in these panels. (C) Replication of VSV minireplicon RNA in the presence of various amounts (indicated in micrograms above each lane) of transfected P_226/227 plasmid. Analysis of replication was performed as described in the legend to Fig. 2. The arrow indicates the negative-sense replication product. The asterisk shows the transcription product which is sometimes nonspecifically immunoprecipitated by anti-VSV antibodies.

Taken together, these results suggest that at least one of the serine residues at positions 226 and 227 must be phosphorylatedto obtain optimal replication activity of the P protein. In addition,the results indicate that Ser-233 does not play any role in thereplication function of the P protein, consistent with the observationthat this residue is not phosphorylated (12).

Transcription activity of the mutant P proteins remains unaffected. We next examined the ability of these mutant proteins to support transcription in vivo. BHK-21 cells infected with vTF7-3were transfected with plasmids encoding 9BN minireplicon RNA andN, L, and wild-type or mutant P proteins. The transfected cellswere then labeled with [³H]uridine and [³H]adenosine in the presence of actinomycin D. Total labeled RNAsisolated from these cells were analyzed by electrophoresis. Synthesisof N $Delta$ L mRNA (Fig. 4) was used as a measure of the transcriptionactivity of the mutant P proteins. The results (Fig. 4) show thatP₂₂₆, P₂₂₇, P₂₃₃, P_226/233, and P_227/233 (lanes 4 to 6, 8, and9) are almost as active as the wild-type P protein (lane 3) intranscription. However, the amount of N $Delta$ L mRNA synthesized bythe P_226/227 (lane 7) and P_226/227/233 (lane 10) mutants was significantlyreduced. A quantitative determination of the levels of transcriptionsuggests that the P_226/227 and P_226/227/233 mutants were 8 and12%, respectively, as active as the wild-type protein (Table 1).

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FIG. 4. Transcription activity of P mutants. BHK-21 cells in 35-mm-diameter six-well plates were infected with vTF7-3 and then transfected with 1.5 µg of pN, 0.5 µg of pL, 2.5 µg of p9BN, and 1.0 µg of pET-P plasmids coding for the wild-type or mutant P proteins. The transfected cells were labeled with [³H]uridine and [³H]adenosine at 16 h posttransfection for 6 h in the presence of actinomycin D. Total RNA from the cytoplasmic extracts was recovered and analyzed by electrophoresis as described in Materials and Methods. G and N represent the corresponding VSV mRNAs isolated from infected cells. The asterisk shows the N $Delta$ L RNA transcription product.

Since the genomic-sense transcription template in our experiment is generated through replication of an antigenomic-senseminireplicon synthesized from the transfected plasmid, the lowlevel of transcription by P_226/227 and P_226/227/233 mutants appearsto be due to low levels of transcription template generated bythese mutants (Fig. 2, lanes 7 and 10, and Table 1). To obtaina more accurate estimation of the relative levels of transcriptionactivity of these mutants, we normalized the levels of transcriptionrelative to the levels of replication as described in Materialsand Methods. In a separate experiment, we first established thatthe amount of transcription, as measured by the synthesis of N $Delta$ LmRNA, directly correlated with the amount of genomic-sense transcriptiontemplate in transfected cells. In this experiment, vTF7-3-infectedcells were transfected with varying amounts of plasmids encodingthe minireplicon RNA along with fixed amounts of plasmids encodingthe N, L, and wild-type P proteins. The cells were metabolicallylabeled with [³H]uridine and [³H]adenosine in the presence of actinomycin D. Replication products(RNAs recovered from immunoprecipitated nucleocapsids) and transcriptionproducts were analyzed by electrophoresis and fluorography andquantitated by densitometric scanning of the fluorograms as describedin Materials and Methods. The results (not shown) demonstrateda linear relationship between the genomic-sense replication product(or transcription template) and the transcription product. Whenthe normalized levels of transcription for various mutant P proteinswere calculated, it was found that all the mutant proteins supportedlevels of transcription comparable to that of the wild-type Pprotein (Fig. 5). These results were consistently obtained infour to five independent experiments. We conclude from these studiesthat phosphorylation of serine residues at positions 226 and/or227 in domain II of the P protein do not play a role in the transcriptionfunctions of the protein.

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FIG. 5. Relative levels of replication and normalized levels of transcription supported by various mutant P proteins. The data were obtained by densitometric scanning of fluorograms as described in Materials and Methods. The histograms represent data from four to five separate experiments, including those shown in Fig. 2, 4, and 6. The average and range of each value are shown.

Substitution of glutamic acid at the phosphate acceptor sites does not rescue optimal replication functions of P protein. One of the consequences of phosphorylation of amino acid residues in a protein is the introduction of negative charges. Wewondered whether phosphorylation per se of the Ser-226 and Ser-227residues of P protein is essential for optimal replication functionsof the protein or whether substitution of negatively charged residuesin place of these serine residues can generate replicationallyactive P protein. To address this possibility, we generated amutant P protein (P_EE) in which serine residues at positions 226and 227 were replaced with glutamic acid residues. The abilityof the mutant protein to support replication of the VSV minigenomewas analyzed. The results (Fig. 6A) show that the P_EE mutant (lane5) is slightly more active in replication than the analine-substitutedmutant protein (lane 4). However, the level of replication supportedby P_EE is only 12 to 14% of that of the wild-type protein (lane3). When the transcription activity of these mutant proteins wasmeasured, P_EE consistently produced slightly higher levels ofN $Delta$ L mRNA (Fig. 6B, lane 5) than P_226/227 (lane 4). This is mostlikely due to higher levels of transcription templates generatedby the P_EE mutant than the P_226/227 mutant. When the level oftranscription was normalized to the amount of transcription template,P_EE was found to be about 90 to 95% as active as the wild-typeP protein (Fig. 5).

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FIG. 6. Replication (A) and transcription (B) supported by P_EE. These experiments were performed as described in the legend to Fig. 2 and 4. The arrow in panel A and the asterisk in panel B show the replication and transcription products, respectively.

These results (Fig. 6) suggest that substitution of negatively charged (glutamic acid) residues at the phosphate acceptorsites does not rescue the optimal replication activity of theP protein. This indicates that phosphorylation of these residuesrather than negative charges in this region is important for thefunction of P protein in replication. The observation that P_EEwas almost as active as P_226/227 or wild-type P in transcriptionfurther confirms that phosphorylation of these residues does notplay any role in P protein function intranscription.

P_226/227 mutant protein acts as an inhibitor of wild-type P protein in replication. We next wanted to determine whether the P_226/227 mutant, which is defective in supporting optimal levels of replication, whencoexpressed along with the wild-type protein, can interfere withthe normal functioning of the wild-type protein in replication.To examine this, replication of the VSV minigenome in transfectedcells coexpressing various amounts of P_wt and P_226/227 proteinswas analyzed. The results from such an experiment (Fig. 7) showthat coexpression of a fixed amount of P_wt and varying amountsof P_226/227 (lanes 6 to 8) led to significant inhibition of minigenomereplication. It must be noted that increasing the amounts of P_wtor P_226/227 led to inhibition of minigenome replication (datanot shown), most likely due to imbalance in the molar amountsof the viral proteins required for replication (46). However,the inhibitory activity of P_226/227 is clearly evident when onecompares levels of replication supported by a given amount ofP_wt with that supported by the same amount of both P_wt and P_226/227.The amount of replication with 4 µg of total plasmids (2 µg eachof P_wt and P_226/227) (Fig. 7, lane 7) was approximately one-thirdof that obtained with 4 µg of P_wt plasmid alone (lane 3). Likewise,the amount of replication with 6 µg of total plasmids (2 µg ofP_wt and 4 µg of P_226/227) (Fig. 7, lane 8) was approximately one-fourthof that obtained with 6 µg of P_wt plasmid alone (lane 4). In addition,when 2 µg of P_wt plasmid was used along with increasing amountsof P_226/227, significant inhibition of replication was observed(compare the levels of replication in Fig. 7, lane 2, with thosein lanes 6 to 8). These results, therefore, indicate that P_226/227protein inhibits the function of P_wt protein in replication invivo.

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FIG. 7. Inhibitory activity of P_226/227 in replication when coexpressed with wild-type P. The value above each lane indicates the amount (in micrograms) of each P plasmid used in the transfection. The experiment was performed as described in the legend to Fig. 2. The arrow shows the replication product.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The phosphoprotein (P) of VSV plays a central role in the transcription and replication functions of the RNA-dependent RNApolymerase of the virion. Although the P protein does not carryany enzymatic activities of the viral polymerase, its interactionwith the large protein, L, generates a specific P-L complex(es)which is absolutely essential for the polymerase activity. TheP protein interacts with soluble N protein to form N-P complexesthat are required for encapsidation of nascent RNA chains duringreplication. P protein is known to exist as oligomers, and oligomerizationof P protein appears to be required for interaction with the Lprotein to generate transcription activity of the P-L complex.In addition, the P protein exists in multiple phosphorylated formswithin the virion core as well as in infected cells, and phosphorylationof residues within specific domains of the P protein regulatesits RNA-synthetic activities. Because of the multifunctional natureof the P protein, a great deal of investigation has been directedtowards understanding its structure-functionrelationships.

We and others have shown recently that phosphorylation of specific residues within domain I of P protein of Indiana serotypeVSV is not essential for the in vivo replication function of theprotein (45, 52). However, in vivo transcription activityof the protein required phosphorylation of the residues in thisdomain (45), although low levels of in vitro transcription activitywere obtained with domain I phosphorylation-defective P protein(52). In the present work, we have examined the role of phosphorylationof domain II residues in in vivo transcription and replicationactivities of the protein. Our results suggest that phosphorylationof a specific serine residue(s) (Ser-226 or Ser-227) in this domainis required for optimal replication activity of the protein. Interestingly,transcription activity of the protein was not adversely affectedby the phosphorylation status of the domain II residues. The majorconclusion that can be drawn from our studies is that phosphorylationat two different domains in the P protein of VSV regulates itsactivity in transcription and replication. However, it must bepointed out that the requirement for phosphorylation of domainI residues in transcription could be overcome by substitutionof negatively charged residues for serine residues (24, 45)whereas appreciable levels of replication could not be rescuedby substitution of glutamic acid residues for serine residuesin domain II (Fig. 6). These results may suggest a unique roleof phosphorylation in the function of the P protein in replicationbut not intranscription.

Recently, it was demonstrated (23) that serine residues at positions 227 and 233 within domain II of P_I are the major targetsof phosphorylation by LAK. However, in a separate study, it wasshown by mutational and biochemical analyses that serine residuesat 226 and 227 are the sites of phosphorylation by LAK (12).The reason(s) for this discrepancy is not clear at this time butthe results of our functional analysis of the mutant P proteins,in which each of these three sites was altered to alanine individuallyor in various combinations, indicate that Ser-233 does not appearto play any role in transcription or replication functions ofthe protein. Our results are consistent with those reported earlierfrom in vitro-transcription studies, suggesting that phosphorylationof domain II residues by LAK has no role in the transcriptionactivity of P_I (23, 40). These results appear to conflictwith those obtained previously, which showed that phosphorylationof Ser-236 and Ser-242 in domain II of P_NJ by LAK is necessaryfor efficient transcription in vitro (11). It is possible thatthe activity of the mutant proteins differs under in vivo andin vitro conditions, as has been demonstrated recently with domainI phosphorylation-defective P mutant proteins (45, 52). Alternatively,it is possible that the functional requirement for phosphorylationof domain II residues of P_NJ may be different from that of P_I.This may be borne out by the observation that phosphorylationof domain I residues of P_NJ is a prerequisite for phosphorylationof domain II residues (4) whereas domain II of P_I can be phosphorylatedwithout prior phosphorylation of domain I residues (12).

The observation that domain II phosphorylation-defective P protein is defective in replication but not in transcription indicatesthat phosphorylation of domain II residues may be important forformation of replicase complexes. We recently suggested that thereplicase complex of VSV may exist as a tripartite complex consistingof the N, P, and L proteins (16) and that other cellular factorsmay also be present in the replicase complex (26). It is possiblethat phosphorylation of domain II residues results in a conformationthat facilitates specific interaction with the L and/or N proteinfor assembly of the replicase complex. The P protein, lackingphosphates in domain II residues, may interact poorly with theother viral proteins so that low levels of replication complexesare formed or that the replication complexes are less active.It is obviously important to examine the interaction of the mutantP proteins with the N and L proteins to understand how phosphorylationin domain II of P might influence the assembly and activity ofthe replicase complex. It must be noted here that the mutant protein(P_227/233) multimerized and interacted well with the L protein(23). However, the data should be considered in the contextthat this mutant protein was phosphorylated at Ser-226 (12).

Several recent studies have provided a correlation between the degree of phosphorylation of the P protein and its activityin transcription and replication. Using okadaic acid, a serine/threoninephosphatase inhibitor, it was shown that the hyperphosphorylatedform of the P protein (presumably having phosphates in both domainI and II residues) inhibited replication (10). Conversely, dephosphorylationof P protein by bacterial alkaline phosphatase (BAP) led to increasedgenome replication, with a concomitant decrease in transcription(49). The amount of BAP needed to stimulate genome replicationand inhibit transcription was substantially below that neededto obtain a noticeable increase in reactivity to a monoclonalantibody (6D11) directed against an epitope that maps to residues177 to 227 of the P protein (49, 55), corresponding to partof domain II. Although these studies did not map the sites fromwhich phosphate moieties were removed by BAP treatment, they indicatedthat the epitope bound by 6D11 antibody is changed by dephosphorylation(49). Since treatment of infected-cell P protein with BAP increasedgenome replication and inhibited transcription without a noticeableincrease in 6D11 antibody reactivity, these results indicate thatBAP may have removed phosphates only from domain I residues. Theseobservations, together with our previous results (45) and thedata presented here, suggest that the P1 protein, with phosphorylationof domain I residues, may function as part of a transcriptioncomplex whereas the P2 protein, with phosphorylation of residuesin domain II, may function exclusively as part of a replicationcomplex. Another subset of P proteins (hyperphosphorylated P2protein with phosphorylation of both domain I and II residues)may be involved in maturation of nucleocapsids for packaging andthereby indirectly inhibit replication (10). Further studiesfocusing on isolation of complexes specific for transcriptionand replication and examination of the phosphorylation statusof P protein in these complexes may provide more direct evidenceas to the role of phosphorylation of residues in various domainsin transcription andreplication.

The inhibitory activity of P_226/227 in replication by wild-type P protein (Fig. 7) indicates that the domain II phosphorylation-defectiveP protein perhaps interacts with the other components of the replicationmachinery to generate inactive complexes or competes with thewild-type P protein for replication machinery. Studies to examinespecific interactions of the mutant protein with the N, L, orN-RNA template may provide a better understanding of the inhibitoryeffect of the mutant protein inreplication.

The phosphate acceptor sites (Ser-226 and Ser-227) within domain II are located adjacent to each other, and our results (Fig.2) show that phosphorylation of either of these two residues issufficient to obtain optimal replication activity of the protein.Furthermore, previous data indicate that phosphorylations at thesesites are independent of each other (12). The question thenis why two functionally redundant phosphorylation sites are maintainedin the protein. It is possible that in a given P molecule, onlyone of these two sites is phosphorylated in vivo and the othersite may remain unphosphorylated because of steric hindrance.Alternatively, the presence of two functionally redundant phosphorylationsites next to each other may protect the protein from becominginactivated in replication by phosphatases, which must removeboth of the phosphate moieties at the sametime.

In summary, the results reported in this article suggest that phosphorylation of either the Ser-226 or Ser-227 residue indomain II is necessary for optimal replication activity, but notfor transcription activity, of the P protein. Substitution ofnegatively charged residues for these residues cannot rescue replication.From these results and those reported previously (10, 23,24, 45, 49, 52), we conclude that phosphorylation withindifferent domains of the P protein controls its activity in transcriptionand replication. Studies of infectious molecular clones of VSVcontaining various phosphorylation-defective mutants of P proteinmay provide additional information as to the role of this modificationin the RNA-synthetic processes of VSV. In several other negative-strandRNA viruses, the P protein has been found to be phosphorylated(5, 7, 14, 17, 19, 42, 43, 54), and the functionalsignificance of phosphorylation in transcription has also beendocumented (5, 7, 17, 42). Whether transcriptase andreplicase activities are regulated by differential phosphorylationof the P proteins of these viruses remains to beexamined.

	ACKNOWLEDGMENTS

We thank Michelle Perez for preparation of the manuscript and Jin-Lian Chen for generating the P mutants. We also thank Merckand Co., Inc., Rahway, N.J., for a gift of actinomycinD.

This investigation was supported by Public Health Service Grants AI 34956 (to A.K.P.) and AI 26585 (to A.K.B.) from the NationalInstitutes of Health. L.N.H. was supported by a predoctoral fellowshipfrom the training grant T32 EY07129 from the National EyeInstitute.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Miami School of Medicine,P.O. Box 016960 (R-138), Miami, FL 33101. Phone: (305) 243-6711.Fax: (305) 243-4623. E-mail: apattnaik{at}mednet.med.miami.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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2. Barik, S., and A. K. Banerjee. 1991. Cloning and expression of the vesicular stomatitis virus phosphoprotein gene in Escherichia coli: analysis of phosphorylation status versus transcriptional activity. J. Virol. 65:1719-1726[Abstract/Free Full Text].

3. Barik, S., and A. K. Banerjee. 1992. Phosphorylation by cellular casein kinase II is essential for transcriptional activity of vesicular stomatitis virus phosphoprotein. Proc. Natl. Acad. Sci. USA 89:6570-6574[Abstract/Free Full Text].

4. Barik, S., and A. K. Banerjee. 1992. Sequential phosphorylation of the phosphoprotein of vesicular stomatitis virus by cellular and viral protein kinases is essential for transcriptional activation. J. Virol. 66:1109-1118[Abstract/Free Full Text].

5. Barik, S., T. McLean, and L. Dupuy. 1995. Phosphorylation of Ser²³² directly regulates the transcriptional activity of the P protein of human respiratory syncytial virus: phosphorylation of Ser²³⁷ may play an accessory role. Virology 213:405-412[Medline].

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7. Byrappa, S., Y.-B. Pan, and K. C. Gupta. 1996. Sendai virus P protein is constitutively phosphorylated at serine 249: high phosphorylation potential of the P protein. Virology 216:228-234[Medline].

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9. Canter, D. M., and J. Perrault. 1996. Stabilization of vesicular stomatitis virus L polymerase protein by P protein binding: a small deletion in the c-terminal domain of L abrogates binding. Virology 219:376-386[Medline].

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1.	Banerjee, A. K., and S. Barik. 1992. Gene expression of vesicular stomatitis virus genome RNA. Virology 188:417-428[Medline].
2.	Barik, S., and A. K. Banerjee. 1991. Cloning and expression of the vesicular stomatitis virus phosphoprotein gene in Escherichia coli: analysis of phosphorylation status versus transcriptional activity. J. Virol. 65:1719-1726[Abstract/Free Full Text].
3.	Barik, S., and A. K. Banerjee. 1992. Phosphorylation by cellular casein kinase II is essential for transcriptional activity of vesicular stomatitis virus phosphoprotein. Proc. Natl. Acad. Sci. USA 89:6570-6574[Abstract/Free Full Text].
4.	Barik, S., and A. K. Banerjee. 1992. Sequential phosphorylation of the phosphoprotein of vesicular stomatitis virus by cellular and viral protein kinases is essential for transcriptional activation. J. Virol. 66:1109-1118[Abstract/Free Full Text].
5.	Barik, S., T. McLean, and L. Dupuy. 1995. Phosphorylation of Ser²³² directly regulates the transcriptional activity of the P protein of human respiratory syncytial virus: phosphorylation of Ser²³⁷ may play an accessory role. Virology 213:405-412[Medline].
6.	Bell, J. C., and L. Prevec. 1985. Phosphorylation sites on phosphoprotein NS of vesicular stomatitis virus. J. Virol. 54:697-702[Abstract/Free Full Text].
7.	Byrappa, S., Y.-B. Pan, and K. C. Gupta. 1996. Sendai virus P protein is constitutively phosphorylated at serine 249: high phosphorylation potential of the P protein. Virology 216:228-234[Medline].
8.	Campbell, M. J. 1995. Lipofection reagents prepared by a simple ethanol injection technique. BioTechniques 18:1027-1032[Medline].
9.	Canter, D. M., and J. Perrault. 1996. Stabilization of vesicular stomatitis virus L polymerase protein by P protein binding: a small deletion in the c-terminal domain of L abrogates binding. Virology 219:376-386[Medline].
10.	Chang, T. L., C. S. Reiss, and A. S. Huang. 1994. Inhibition of vesicular stomatitis virus RNA synthesis by protein hyperphosphorylation. J. Virol. 68:4980-4987[Abstract/Free Full Text].
11.	Chattopadhyay, D., and A. K. Banerjee. 1987. Phosphorylation within a specific domain of the phosphoprotein of vesicular stomatitis virus regulates transcription in vitro. Cell 49:407-414[Medline].
12.	Chen, J.-L., T. Das, and A. K. Banerjee. 1997. Phosphorylated states of vesicular stomatitis virus P protein in vitro and in vivo. Virology 228:200-212[Medline].
13.	Clinton, G. M., and A. S. Huang. 1981. Distribution of phosphoserine, phosphothreonine, and phosphotyrosine in proteins of vesicular stomatitis virus. Virology 108:510-514[Medline].
14.	Curran, J., T. Pelet, and D. Kolakofsky. 1994. An acidic activation-like domain of the Sendai virus P protein is required for RNA synthesis and encapsidation. Virology 202:875-884[Medline].
15.	Das, T., A. K. Gupta, P. W. Sims, C. A. Gelfand, J. E. Jentoft, and A. K. Banerjee. 1995. Role of cellular casein kinase II in the function of the phosphoprotein (P) subunit of RNA polymerase of vesicular stomatitis virus. J. Biol. Chem. 270:24100-24107[Abstract/Free Full Text].
16.	Das, T., A. K. Pattnaik, A. M. Takacs, T. Li, L. N. Hwang, and A. K. Banerjee. 1997. Basic amino acid residues at the carboxy-terminal eleven amino acid region of the phosphoprotein (P) are required for transcription but not for replication of vesicular stomatitis virus genome RNA. Virology 238:103-114[Medline].
17.	Das, T., A. Schuster, S. Schneider-Schaulies, and A. K. Banerjee. 1995. Involvement of cellular casein kinase II in the phosphorylation of measles virus P protein: identification of phosphorylation sites. Virology 211:218-226[Medline].
18.	De, B. P., and A. K. Banerjee. 1985. Requirements and functions of vesicular stomatitis virus L and NS proteins in the transcription process in vitro. Biochem. Biophys. Res. Commun. 26:40-49.
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20.	Emerson, S. U., and Y. H. Yu. 1975. Both NS and L proteins are required for in vitro RNA synthesis by vesicular stomatitis virus. J. Virol. 15:1348-1356[Abstract/Free Full Text].
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