Persistent Activation of RelA by Respiratory Syncytial Virus Involves Protein Kinase C, Underphosphorylated Ikappa Bbeta , and Sequestration of Protein Phosphatase 2A by the Viral Phosphoprotein

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J Virol, July 1998, p. 5610-5618, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Persistent Activation of RelA by Respiratory Syncytial Virus Involves Protein Kinase C, Underphosphorylated I $kappa$ B $beta$ , and Sequestration of Protein Phosphatase 2A by the Viral Phosphoprotein

Vira Bitko and Sailen Barik^*

Department of Biochemistry and Molecular Biology, College of Medicine, University of South Alabama, Mobile, Alabama 36688-0002

Received 14 January 1998/Accepted 24 March 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Respiratory syncytial virus (RSV) activated the RelA (p65) subunit of nuclear factor kappa B (NF- $kappa$ B) over many hours postinfection.The initial activation coincided with phosphorylation and degradationof I $kappa$ B $alpha$ , the cytoplasmic inhibitor of RelA. During persistentactivation of NF- $kappa$ B at later times in infection, syntheses ofinhibitors I $kappa$ B $alpha$ as well as I $kappa$ B $beta$ were restored. However, the resynthesizedI $kappa$ B $beta$ was in an underphosphorylated state, which apparently preventedinhibition of NF- $kappa$ B. Use of specific inhibitors suggested thatthe pathway leading to the persistent $---$ but not the initial $---$ activationof NF- $kappa$ B involved signaling through protein kinase C (PKC) andreactive oxygen intermediates of nonmitochondrial origin, whereasphospholipase C or D played little or no role. Thus, RSV infectionled to the activation of NF- $kappa$ B by a biphasic mechanism: a transientor early activation involving phosphorylation of the inhibitorI $kappa$ B polypeptides, and a persistent or long-term activation requiringPKC and the generation of hypophosphorylated I $kappa$ B $beta$ . At least apart of the activation was through a novel mechanism in whichthe viral phosphoprotein P associated with but was not dephosphorylatedby protein phosphatase 2A and thus sequestered and inhibited thelatter. We postulate that this led to a net increase in the phosphorylationstate of signaling proteins that are responsible for RelA activation.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Human respiratory syncytial virus (RSV) is the leading cause of respiratory illness and death in young infants worldwide (3,29). It is the prototype member of the genus Pneumovirus inthe family Paramyxoviridae and contains a nonsegmented negative-strandRNA genome about 15 kb long (6, 17). Due to the profoundclinical importance of the virus and the lack of a reliable vaccine,new lines of investigation have placed much emphasis on host-virusinteractions in relation to the immunopathology of the infectionprocess. Recent studies have demonstrated the elaboration of anumber of cytokines and other immunoregulatory molecules followingRSV infection of a variety of susceptible host cells of the respiratorytract. These products include but are not limited to leukotrienes(2), intracellular adhesion molecule-1 (43, 51), majorhistocompatibility class I molecule (25), soluble tumor necrosisfactor (TNF) receptor (5), and a battery of interleukins andchemokines, such as interleukin-1 (IL-1), IL-6, IL-8, IL-10, andIL-11 (11-13, 20-23, 26, 38, 42, 45). In order to addressthe mechanism underlying the activation of these cytokines, suchstudies have been extended to RSV infection of defined and establishedcell lines of lung origin. RSV infection of A549 cells, in particular,has been shown to result in the induction of essentially all ofthe interleukins mentioned above (13, 23, 25, 26, 38,43).

Others and we have recently demonstrated that RSV infection leads to the activation of cellular transcription factor NF- $kappa$ B,which is in turn responsible for transcriptional activation ofa number of interleukin promoters (13, 22, 26, 38). RSVinfection was shown to induce nuclear translocation of the existingRelA subunit and to a lesser extent the p50 subunit of NF- $kappa$ B overmany hours postinfection (p.i.). A large body of recent literaturehas established a relatively detailed mechanism of NF- $kappa$ B inductionthat can occur in response to various extracellular signals (reviewedin references 10, 37, 48, and 50). In the uninduced cell,NF- $kappa$ B is retained in the cytoplasm in complex with its inhibitorysubunit, I $kappa$ B $alpha$ , which is believed to mask the nuclear localizationsequence (NLS) of NF- $kappa$ B. One of the earliest discernible biochemicalreactions in the NF- $kappa$ B activation pathway is the phosphorylationof I $kappa$ B $alpha$ by a novel multisubunit kinase complex (27, 37, 50),followed by their degradation, most likely by the ubiquitin-proteasomepathway (15). This leads to nuclear translocation of NF- $kappa$ B,which then activates a variety of cellular genes, including thoseof many interleukins and I $kappa$ B. Following the initial activation,NF- $kappa$ B therefore produces new rounds of I $kappa$ B $alpha$ which restores inhibition,thus generating an autoregulatory loop, which explains the transientinduction of NF- $kappa$ B by signals such as TNF- $alpha$ and phorbol esters.This mechanism, however, fails to explain the persistent inductionof NF- $kappa$ B by lipopolysaccharides and IL-1, which lasts for manyhours following stimulation. Recent studies have suggested a rolefor another inhibitor, I $kappa$ B $beta$ , in this process (44, 54). Thenewly synthesized I $kappa$ B $beta$ , which was found to be underphosphorylated,was shown to complex with NF- $kappa$ B; however, unlike I $kappa$ B $alpha$ , it apparentlydid not mask the NLS of NF- $kappa$ B. Additionally, it prevented I $kappa$ B $alpha$ from binding to NF- $kappa$ B. Thus, the transcriptionally competent NF- $kappa$ B-I $kappa$ B $beta$ complex entered the nucleus and functioned essentially like activatedNF- $kappa$ B. Although the kinetic details of the interaction betweenthe two forms of I $kappa$ B with the various subunits of NF- $kappa$ B remainto be elucidated, this model offers a plausible mechanism forpersistent induction over long periods.

As alluded to earlier, activation of the NF- $kappa$ B RelA (p65) subunit by RSV was found to be clearly persistent in nature (13,26) (Fig. 1). Here, we report a potential mechanism for thisinduction and show that the signal transduction pathway leadingto it involves protein kinase C (PKC) enzyme(s) that apparentlygenerates reactive oxygen of potentially nonmitochondrial origin.This in turn leads to phosphorylation and degradation of I $kappa$ B proteins,and eventual generation of newly synthesized underphosphorylatedI $kappa$ B $beta$ , thus leading to persistent induction. Interestingly, theviral phosphoprotein P alone caused substantial activation ofRelA through an apparently novel mechanism. It was not a substrateof cellular phosphatases; nevertheless, it did bind protein phosphatase2A (PP2A) and thus sequestered, and essentially inhibited, thelatter. We propose that the inhibition of PP2A leads to increasedphosphorylation of specific cellular proteins, some of which aresignaling molecules in the RelA activation pathway.

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FIG. 1. Kinetics of RelA activation by RSV. Infection of A549 cells by RSV, preparation of nuclear (Nucl) and cytoplasmic (Cyto) extracts, and determination of RelA levels by immunoblotting were performed as described in Materials and Methods. At various times p.i., cells were harvested for lysis: lane 1, 0 h; lane 2, 2 h; lane 3, 4 h; lane 4, 6 h; lane 5, 8 h; lane 6, 10 h; lane 7, 20 h; lane 8, 30 h; lane 9, 10 h; lane 10, 30 h. ECL immunoblot analyses of cytosolic and nuclear fractions (as indicated) were carried out with anti-p65 antibody.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Antibodies and inhibitors. Rabbit antipeptide antibodies made against epitopes of RelA (p65), I $kappa$ B $alpha$ , and I $kappa$ B $beta$ were purchased from Santa Cruz Biotechnology(Santa Cruz, Calif.). Antibodies against the catalytic subunitsof PP1 and PP2A were purchased from Transduction Laboratories(Lexington, Ky.). Calyculin A, rotenone, sodium orthovanadate,sphingosine, and pyrrolidone dithiocarbamate (PDTC) were fromSigma Chemical Co. (St. Louis, Mo.); D609 and U73122 were fromBIOMOL Research Laboratories (Plymouth Meeting, Pa.); MG132 (Z-Leu-Leu-Leu-CHO)was from Peptide Institute (Osaka, Japan); and Myr- $psi$ PKC (myr.Arg-Phe-Ala-Arg-Lys-Gly-Ala-Leu-Arg-Gln-Lys-Asn-Val),a pseudosubstrate peptide that is cell permeable due to its myristyl(myr.) group and inhibits PKC, was from Promega Corp. (Madison,Wis.). The lambda phosphatase (PP $lambda$ ) was purified as describedpreviously (8); the catalytic subunit of PP2A and cyclic AMP-dependentprotein kinase (PKA) were purchased from Promega. Stock solutions(200× to 500×) of the inhibitor chemicals (for example, okadaicacid [OA]) were made in water or dimethyl sulfoxide as instructedby the manufacturer. Unless otherwise mentioned, the inhibitorswere added to RSV-infected cells at 3 h after addition of thevirus and at the final concentrations indicated for each experiment.Anti-RSV antibody was purchased from Chemicon International, Inc.(Temecula, Calif.).

Estimation of RSV growth. The growth of RSV (Long) in A549 cells in the presence or absence of various drugs was quantitated by either of the following,as and where mentioned: determination of viral titer on HEp-2monolayers by standard procedures, immunoprecipitation of [³⁵S]methionine-labeled RSV proteins as described elsewhere (7),and immunoblotting (Western blotting) of the total infected cellextract with an anti-RSV antibody.

Measurements of NF- $kappa$ B and I $kappa$ B. RSV (Long) inoculum was grown in HEp-2 cells and purified as described earlier (13). For the NF- $kappa$ B experiments, monolayersof A549 cells were infected with purified RSV at a multiplicityof infection (MOI) of 3.0. Inhibitor drugs at appropriate concentrationswere added 1.5 h after the addition of the virus. The time ofaddition of the virus was considered as 0 h; at specified timesafterward, the infected cells were processed for analysis essentiallyas described above. Briefly, the infected monolayer (and the uninfectedcontrol) was washed twice with ice-cold phosphate-buffered saline.Then 500 µl of lysis buffer (50 mM Tris-Cl [pH 8.0], 50 mM NaCl,0.1 mM EDTA, 1% Tween 20, 1 mM dithiothreitol, leupeptin, aprotinin,phenylmethylsulfonyl fluoride) was added per 150-cm² T flask, and the mixture was incubated for 10 min at room temperature.The lysed cells were scraped off, and the extract was centrifugedat 2,000 × g for 5 min. The supernatant was further clarifiedby centrifugation at 15,000 × g for 15 min in cold and was usedas cytosolic extract in immunoblot analysis where mentioned. Thepellet, containing nuclei, was washed twice with 500 µl of ice-coldlysis buffer. Both fractions were either immediately used in immunoblotanalysis or stored frozen at $-$ 80°C until use.

Immunoblot analyses were carried out with antibodies against RelA (p65), I $kappa$ B $alpha$ , and I $kappa$ B $beta$ , purchased from Santa Cruz Biotechnology;15 µg of the nuclear (for RelA) extract or 30 µg of cytosolicextract (for I $kappa$ B and P proteins) was analyzed on 14% denaturingpolyacrylamide gels. To achieve a good separation of the phosphorylatedand basal forms of I $kappa$ B $beta$ , such gels were made in a 10-in.-tallgel apparatus, and electrophoresis was carried out at a constant100 V overnight. Following electrophoresis, the proteins wereelectroblotted to Immobilon-P (Millipore) membranes. Blockingand probing of the membranes and development of the bands by enhancedchemiluminescence (ECL; Amersham) were performed essentially asdescribed previously (39).

Electrophoretic mobility shift assays (EMSA) using nuclear extracts (19) of RSV-infected cells and double-stranded ³²P-labeled NF- $kappa$ B oligonucleotide (5' GGGGAATTTCCCC 3') were carriedout as described earlier (13).

Functional assays of NF- $kappa$ B activity were performed in A549 cells transfected with the NF- $kappa$ B monitor plasmid pBIIxluc followedby infection with RSV and luciferase assays, essentially as describedpreviously (13, 33).

Immunoprecipitation. A549 cells, grown in 10-cm-diameter dishes to a confluency of 70%, were transfected with pcDNA-3 clones of wild-type or mutantP genes of RSV as described earlier (9). Preparation of cellextracts and immunoprecipitation using either anti-P or anti-PP2Aantibodies and protein A-coupled Sepharose beads were performedas described previously (9). The anti-P antibody was raisedin rabbits against peptide CSDNPFSKLYKETIETFD (residues 94 to110 of the P protein of Long strain with a cysteine added to theN terminus) by conjugation with keyhole limpet hemocyanin accordingto standard procedures.

Phosphatase assays. Phosphatase activities were assayed in standard 20-µl reaction mixtures containing 50 mM Tris-Cl (pH 7.5), 50 mM NaCl, 5 mMMgCl₂, 5 mM MnCl₂, 100 µM ATP (to reduce the specific activityof any [ $gamma$ -³²P]ATP that might be carried over from the previous phosphorylationreaction), approximately 10 ng of recombinant human PP2A, andeither 20 mM p-nitrophenyl phosphate (pNPP) or 0.5 µg of ³²P-labeled casein or histone as the substrate, essentially as describedpreviously (4). The hydrolysis of pNPP was quantitated by acolorimetric assay; that of casein or histone was quantitatedby measuring the liberated inorganic phosphate (4). Caseinand histone were phosphorylated by the catalytic subunit of PKA,using [ $gamma$ -³²P]ATP as the phosphate donor (4), followed by removal of theATP by filtration chromatography through Sephadex G-50. Wherementioned, a variable amount of the phosphorylated or phosphate-freeP protein was also included in the PP2A reaction. PhosphorylatedP protein was prepared in a similar manner by phosphorylatingthe bacterially expressed phosphate-free P protein with caseinkinase 2 (CK2) in vitro (4, 9, 39).

Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) analysis was carried out by the Laemmli procedure (34)as described earlier (39).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Persistent activation of RelA by RSV. To investigate the mechanism of induction of NF- $kappa$ B by RSV, we needed to first determine the kinetics of the induction andthe relationship between the cytoplasmic and the nuclear concentrationsof NF- $kappa$ B. To accomplish this, we isolated the nuclei and cytosolicfractions of A549 cells infected with RSV (MOI of 2.0) at differenttimes p.i. and probed them with anti-RelA antibody in immunoblotanalysis. Results presented in Fig. 1 demonstrate the followingmajor features of the activation process. (i) An increase in thenuclear RelA was accompanied by a parallel decrease in cytoplasmicRelA concentrations, confirming earlier results (26). Thus,the total quantity of RelA polypeptides in the infected cell remainednearly unchanged during induction, except for a small increasebeyond 10 h p.i. (ii) This finding also suggested that at leastat the earlier times, activation of RelA probably involved theclassic mechanism of translocation of preexisting cytoplasmicpool of RelA into the nucleus, pointing to a posttranslationalmodification. A continuous turnover of both cytoplasmic and nuclearpools at later times cannot be excluded at this point. (iii) Translocationseemed to begin as early as 6 h p.i. and reached its maximal levelby 10 to 12 h under the conditions of this experiment. (iv) Perhapsmost interestingly, the elevated nuclear RelA concentration wasmaintained essentially through the whole phase of intracellularmultiplication of the virus, tested up to at least 30 h, whichconfirmed and extended earlier findings (13) and clearly establishedthe persistent nature of RSV-mediated RelA induction. As expected,translocation of RelA was not seen in A549 cells mock infectedwith virus-free supernatants.

RSV-mediated phosphorylation and degradation of I $kappa$ B subunits. To further elucidate the steps in RSV-mediated NF- $kappa$ B induction, we decided to determine the quantity as well as the phosphorylationstatus of the two I $kappa$ B proteins during induction. Increased phosphorylationof the I $kappa$ Bs has been shown to result in their slower mobilityin denaturing polyacrylamide gels (54). Thus, to determine whetherphosphorylation of the I $kappa$ Bs is induced by RSV, the total-cellextracts of RSV-infected cells were electrophoresed such thatthe phosphorylated forms of the I $kappa$ B proteins were resolved fromtheir nonphosphorylated (or underphosphorylated) forms. The gelwas then subjected to standard immunoblot analysis using anti-I $kappa$ Bantibodies as described in Materials and Methods. Results presentedin Fig. 2 clearly show that both I $kappa$ B $alpha$ and I $kappa$ B $beta$ were found in uninfectedA549 cells. Soon after RSV infection, both I $kappa$ Bs rapidly disappeared(lanes 3 and 4). For I $kappa$ B $alpha$ , an intermediate, more slowly migratingform could be detected, suggesting a causal relationship betweenRSV-induced phosphorylation and degradation. The more highly phosphorylatednature of the more slowly migrating forms of both I $kappa$ Bs could bejudged by their disappearance (Fig. 2, lane W) upon treatmentwith PP $lambda$ , a Ser/Thr protein phosphatase of broad specificity (4,8, 9). The dephosphorylation was not seen in the presenceof sodium orthovanadate, a potent inhibitor of PP $lambda$ (data not shown),or when a phosphatase-defective mutant of PP $lambda$ (Asp20 to Asn [4])was used (Fig. 2, lane M), demonstrating that the disappearanceof the more slowly migrating band upon phosphatase treatment wasnot due to a nonspecific protease present in the phosphatase preparation.In contrast to I $kappa$ B $alpha$ , I $kappa$ B $beta$ clearly existed in a constitutivelyphosphorylated state in uninfected cells (Fig. 2B, lane 1). Inour gel conditions, we could not detect its additional phosphorylation;thus, further studies are needed to ascertain a possible RSV-inducedphosphorylation of I $kappa$ B $beta$ that would serve as a signal for its subsequentdegradation.

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FIG. 2. Time course of phosphorylation and degradation of I $kappa$ B $alpha$ (A) and I $kappa$ B $beta$ (B). ECL immunoblot analyses of total extracts of RSV-infected (and control, mock-infected) A549 cells were carried out with anti-I $kappa$ B $alpha$ and -I $kappa$ B $beta$ antibodies as described in Materials and Methods. The time points of harvest were as in Fig. 1. Cell extracts corresponding to lane 3 of panel A or lane 2 of panel B were incubated with 1 µg of wild-type (lane W) or mutant (lane M) PP $lambda$ in the presence of 4 mM MnCl₂ at room temperature for 2 min before being subjected to SDS-PAGE; 20 µg protein was analyzed in each lane, except lane M in panel B, for which 40 µg was used.

Regardless of its exact mechanism, the onset of the degradation of I $kappa$ Bs (about 6 h p.i.) correlated well with the nucleartranslocation of RelA, as observed in Fig. 1. At later times inRSV infection, however, much of the I $kappa$ B $alpha$ and even more of I $kappa$ B $beta$ reappeared (about 12 h p.i. onward) and continued to be maintainedthroughout the rest of the infection, which is in agreement withthe fact that transcription of both genes is activated by NF- $kappa$ B(10, 48). The newly synthesized I $kappa$ B $beta$ was clearly unphosphorylated,as judged by its faster mobility on SDS-PAGE (Fig. 2B, lanes 4through 8). Thus, it appears that RSV, like cellular agonists,induces the degradation of the I $kappa$ Bs through a net increase intheir phosphorylation (10, 48) and leads to persistent activationNF- $kappa$ B through resynthesized hypophosphorylated I $kappa$ B $beta$ (44, 54).

Requirement of PKC and unphosphorylated I $kappa$ B $beta$ in RSV-mediated activation of NF- $kappa$ B. A number of studies have recently attempted to delineate the signal transduction pathway leading to the activation of NF- $kappa$ B.Briefly, various extracellular signals seemed to activate a PKCor a phospholipase pathway, either of which eventually producedreactive oxygen intermediates (ROIs) as a common intracellularmessenger (summarized in references 10 and 48). In supportof this view, inhibitors of either PKC or phospholipase C (PLC)inhibited activation of NF- $kappa$ B in different systems. Compoundsthat inhibited mitochondrial ROI synthesis, such as amytol androtenone, also inhibited NF- $kappa$ B activation. Finally, a great varietyof antioxidants were reported to suppress the activation of NF- $kappa$ B;notable among these were glutathione, 2-mercaptoethanol, dithiocarbamates,and vitamin E (10). To determine whether similar pathways areoperative in RSV-mediated activation of NF- $kappa$ B, we added variousinhibitors to RSV-infected A549 cells at 2 h p.i. and, at varioustimes afterward, examined the nuclear translocation of RelA, theability of nuclear RelA to bind NF- $kappa$ B DNA elements, and the statusof the I $kappa$ B $alpha$ and $beta$ polypeptides.

To start, we tested the effects of three PLC inhibitors, D609, U73122, and sphingosine. As shown in Fig. 3A, D609 treatmentstrongly inhibited the NF- $kappa$ B activity as measured in EMSA in vitro,while U73122 or sphingosine (data not shown) had no effect. Noneof the PLC inhibitors, including D609, inhibited the nuclear translocationof RelA (Fig. 3B), measured at either 8 or 30 h p.i.; therefore,only the D609 data are shown as representative. The two PKC inhibitors,staurosporine and the pseudosubstrate peptide (Myr- $psi$ PKC), bothstrongly inhibited DNA-binding activity (Fig. 3A) as well as nucleartranslocation (Fig. 3B) of RelA at 30 h p.i. only. Rotenone, aninhibitor of mitochondrial synthesis of reactive oxygen, had verylittle effect on either the quantity or activity of nuclear RelA.However, the antioxidant PDTC did inhibit RelA activation by RSVat both time points, and so did MG132, a proteasome inhibitor,although the effect of the latter was more modest. Based on theseresults, it appears that the drugs that inhibited RelA are oftwo kinds: the PKC inhibitors affected mainly the persistent orlong-term activation of RelA, whereas MG132 and PDTC inhibitedthe persistent as well as the early phases.

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FIG. 3. Effect of signal transduction inhibitors on RSV-mediated activation of NF- $kappa$ B. The inhibitors were added to RSV-infected A549 cells at the following final concentrations: D609, 20 µM; staurosporine (Stau.), 20 ng/ml; pseudosubstrate peptide (Pept.), 100 µM; PDTC, 40 µM; rotenone (Roten.), 40 µM; MG132, 80 µM; and U73122, 30 µM. Numbers above the lanes indicate the hours p.i. at which the cells were harvested for preparing extracts as described in Materials and Methods. (A) EMSA for NF- $kappa$ B-binding activity in nuclear extracts; (B to D) immunoblots of nuclear RelA (B), I $kappa$ B $alpha$ (C), and I $kappa$ B $beta$ (D). The phosphorylated and nonphosphorylated forms of I $kappa$ B polypeptides are indicated. To study the effect of inhibitors on NF- $kappa$ B activity ex vivo, A549 cells were transfected with plasmid pBIIxluc, using Lipofectamine (Gibco-BRL), and then infected with RSV (or mock infected as a control) essentially as described elsewhere (13). The inhibitors were added at 2 h after addition of the virus. At 20 h thereafter, cells were processed for luciferase assay (13). Luciferase activities, expressed as percentages of the untreated activity (E), represent averages of three measurements.

To explore the mechanism of RelA activation further, the effects of these same inhibitors on the status of the I $kappa$ B- $alpha$ and - $beta$ polypeptides were tested by using specific antibodies. Resultspresented in Fig. 3C and D reveal that following the initial degradationat 8 h p.i., substantial quantities of I $kappa$ B $alpha$ reappeared by 30 hp.i. in essentially all cases regardless of the nature of theinhibitor. It is notable that in the case of PDTC and MG132, incontrast to the other inhibitors, more I $kappa$ B $alpha$ escaped degradationat 8 h p.i., which may explain the inhibitory effect of thesetwo drugs on the early activation of RelA as well (Fig. 3A andB). Rotenone, which did not inhibit RelA activation, was includedas a control in these experiments. Based on their slower mobility,the large fraction of undegraded I $kappa$ B $alpha$ and I $kappa$ B $beta$ found in MG132-treatedcells was judged to be phosphorylated. As observed in Fig. 3,MG132 was only partially effective in inhibiting the proteolysisof the I $kappa$ Bs, which correlates with its modest inhibitory effecton RelA activation. The most obvious mechanistic commonality ofthe drugs that did abrogate RelA activation (viz., PDTC, MG132,and the PKC inhibitors) was that they all strongly inhibited thereappearance of I $kappa$ B $beta$ , thus reinforcing a critical role of theunderphosphorylated resynthesized I $kappa$ B $beta$ in the persistent activationof RelA by RSV.

To determine whether the DNA-binding activities determined in EMSA reflect true NF- $kappa$ B transcription activity ex vivo, we testedthe effect of these drugs on the NF- $kappa$ B-dependent expression ofreporter luciferase enzyme from the plasmid pBIIxluc as describedearlier (33). The ex vivo activities of NF- $kappa$ B under the effectof these drugs (Fig. 3E) closely paralleled the DNA-binding activityin EMSA (Fig. 3A).

Taken together, these results lead to the following immediate conclusions. First, RSV effects the persistent activation ofRelA through PKC and reactive oxygen; PLC is not involved in thisactivation, although a D609-sensitive isozyme may play an indirectrole in RelA function. Second, reappearance of I $kappa$ B $alpha$ required activeNF- $kappa$ B; D609 and PDTC inhibited both. Finally, persistent activationby RSV generally correlated with the reappearance of I $kappa$ B $beta$ , whichmost likely served to protect RelA from the newly synthesizedI $kappa$ B $alpha$ .

Intracellular expression of RSV phosphoprotein activates RelA. In a preliminary attempt to identify potential RSV gene products that may be responsible for the activation of NF- $kappa$ B, we decidedto test if intracellular expression of recombinant P protein ofRSV might activate RelA. A549 cells were transfected with theavailable pcDNA3 clone of P (Long strain), and the status of RelAin the transfected cells was determined. The P clone was earliershown to produce P protein in transfected cells, which was phosphorylatedmostly at Ser²³² and to a smaller extent at Ser²³⁷ (9, 39, 46). Results in Fig. 4A show that the recombinantP protein produced a modest but appreciable increase in nuclearRelA protein. The biological activity of RelA was ascertainedby two criteria that we have used earlier: EMSA (Fig. 4B) andproduction of luciferase from the NF- $kappa$ B-dependent reporter plasmidpBIIxluc (Fig. 4C). The authenticity of the role of NF- $kappa$ B wasfurther confirmed by inhibition of luciferase synthesis by sodiumsalicylate (13, 33). Interestingly, expression of a deletionmutant of P missing the C-terminal 39 amino acids that includedthe phosphorylation sites Ser²³² and Ser²³⁷ failed to activate RelA in all these experiments. Two P clones(T1 and T2), in which the third and fourth codons, respectively,of the P gene were mutated to termination codon TAA, also failedto activate RelA (Fig. 4C), suggesting the activation was likelya property of the P protein itself and not due to its mRNA orDNA sequence. Cells transfected with control pcDNA3 vector didnot show any increase in nuclear RelA concentration or activity(Fig. 4B and C). To eliminate the possibility that salicylatehad affected the expression of recombinant P protein, we monitoredthe P protein levels by immunoblot analysis. As shown in Fig.4D, P protein levels in salicylate-treated cells were comparableto those in untreated cells. Thus, we conclude that the recombinantP protein can activate RelA in the absence of any other viralgene product(s). It appeared, however, that the degree of activationwas lower than that seen in RSV-infected cells.

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FIG. 4. Activation of RelA by recombinant RSV P protein. A549 cells at 75% confluency were transfected with pcDNA3-P alone (A, B, and D) or together with pBIIxluc (C) in multiple dishes and processed as indicated, using procedures described in Materials and Methods. The various pcDNA-3 plasmids are vector (V), full-length P clone (P), $Delta$ C39 P clone ( $Delta$ P), and P clones with premature termination codons (T1 and T2). RelA and P protein levels were measured by immunoblotting of nuclear and cytoplasmic fractions, respectively (A and D). NF- $kappa$ B activities in nuclear extracts were assayed by EMSA (B). Ex vivo activities of NF- $kappa$ B were determined by reporter luciferase assay (C); average values from three experiments are shown with standard deviation bars. Where indicated, sodium salicylate (15 mM in panels A and B; 2 and 8 mM in panel C) was added to the transfected cells 4 h after addition of the DNA.

Inhibition of PP2A by RSV phosphoprotein. We have shown earlier that the RSV phosphoprotein is resistant to dephosphorylation by cellular phosphatases in vitro as wellas ex vivo (9). However, it could be dephosphorylated in vitroby the more promiscuous Ser/Thr phosphatase encoded by bacteriophagelambda (4), suggesting that the phosphate groups of the P proteinprobably fail to interact with the catalytic pocket of the eukaryoticphosphatases in a proper manner. Thus, to explain activation ofRelA by P, we entertained the scenario that the P protein maystill bind to eukaryotic phosphatases and thus inactivate thelatter, which in turn would lead to higher levels of cellularphosphorylation leading to activation of RelA. Marine toxins suchas OA and calyculin have been indeed shown to activate RelA whenadded to cell cultures at concentrations that inhibit PP2A morestrongly than PP1 or PP2B (30, 49, 52). To test whetherP protein might function through a similar mechanism, we testedwhether P can inhibit purified human PP2A in vitro. First, weconfirmed that ³²P-labeled P protein is indeed resistant to dephosphorylation bypurified PP2A in vitro (Fig. 5A) although it could be dephosphorylatedby PP $lambda$ . The effect of unlabeled phosphorylated P was then testedon the activity of PP2A, using ³²P-labeled casein as the substrate. The results show that phosphorylatedP protein did inhibit PP2A activity and that phosphate-free Pprotein at similar concentrations was considerably less inhibitory(Fig. 5B and C). Essentially similar conclusions were reachedin assays using phosphohistone as the substrate (data not shown).

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FIG. 5. (A) Resistance of RSV P protein to PP2A. Bacterially expressed RSV P protein was phosphorylated by CK2 in the presence of [ $gamma$ -³²P]ATP (9, 39); 2 µg of the labeled P protein was incubated with 20 ng of purified enzyme (Enz.) PP $lambda$ or PP2A in 20-µl reaction mixtures under standard conditions (4). At the indicated time points, 4 µl of the reaction mixtures was removed and added to 20 µl of Laemmli sample buffer (34). All samples were heated in a boiling water bath for 5 min and analyzed by SDS-PAGE (39) followed by autoradiography as shown. (B and C) Inhibition of PP2A by phosphorylated P protein. Standard phosphatase reactions (20 µl) were carried out with 2 µg of ³²P-labeled casein as the substrate and 4 µg of phosphate-free (P) or phosphorylated (P-PO₄) RSV P protein. At indicated times, 4 µl of the reaction mixture was removed. Reactions were analyzed by SDS-PAGE (34) and autoradiography (B). The multiple bands of ³²P-casein in each lane were scanned by densitometry, and their total intensities were plotted as percentages of the starting intensities (at 0 min) (C). Results are shown for assays with no P added ( $square$ ), unphosphorylated P ( $open circle$ ), and phosphorylated P ( $bullet$ ).

To determine whether P may inhibit PP2A in RSV-infected cells, we took advantage of the facts that the peptide RRREEETEEEAA,phosphorylated at the Thr residue (by CK2 in vitro), is a relativelyspecific substrate of PP2A and that OA at a concentration of 2nM preferentially inhibits the PP2A class of phosphatases. Thus,the specific activity of PP2A in RSV-infected A549 extracts wasquantitated by assaying the OA-sensitive phosphatase activityand comparing it with similar activity in extracts of uninfectedcells. These results revealed a 50 to 60% drop of PP2A activityin the infected cells (data not shown), although it was not possibleto confirm that this was specifically due to the P protein andnot due to any other viral gene product.

RSV phosphoprotein associates with PP2A. To test directly whether RSV P indeed binds to PP2A ex vivo, we transfected A549 cells with the pcDNA3-P clone, immunoprecipitatedthe expressed P protein with a specific anti-P antibody, and thentested for the presence of phosphatases in the precipitate byimmunoblot analysis using antibodies against PP1, PP2A, and PP2B.While no PP1 or PP2B could be detected (data not shown), substantialamounts of PP2A were found in the immunoprecipitates (Fig. 6A).In the reciprocal experiment, immunoprecipitates obtained withanti-PP2A also contained P protein (Fig. 6A). The C-terminal deletionmutant of P, lacking the phosphorylation domain, associated withPP2A to a much lesser extent, although it was expressed as abundantlyas the wild type. Addition of sodium salicylate to the cells hadno effect on the association (data not shown). Association ofP with PP2A, perhaps to a somewhat lesser extent, was also observedin RSV-infected cells (Fig. 6B). Together, these results suggestthat P protein specifically associates with PP2A and that thephosphate groups of P may have a role in stabilizing the association.

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FIG. 6. Association of recombinant (A) and viral (B) P proteins with PP2A. A549 cells were transfected with plasmid pcDNA3-P (lane P), pcDNA3 clone of a $Delta$ C39 deletion mutant of P (lane $Delta$ P), or pcDNA3 vector without P gene (lane V) (A) or infected with RSV (Long) at an MOI of 3.0 (B). At 48 h posttransfection (or p.i.), the cells were processed for immunoprecipitation (IP) using antibodies against either PP2A or RSV P protein as indicated. The samples were analyzed by SDS-PAGE in which the immunoprecipitate from about 10⁶ cells was applied in each lane. The proteins were transferred to a membrane and probed with the same antibodies in Western blot analysis as shown.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this report, we have attempted to delineate the pathway leading to the persistent activation of NF- $kappa$ B by RSV. The principalparticipants in the activation of the RelA subunit of NF- $kappa$ B were(i) viral gene products acting as the proximal signal(s) of activation,at least one of which is the phosphoprotein P functioning throughthe sequestration and inhibition of cellular PP2A and thus likelyincreasing the net phosphorylation of phosphoproteins involvedin the RelA activation pathway; (ii) a D609-sensitive enzyme $---$ perhapssome form of phospholipase $---$ that may positively regulate gene transcriptionby RelA rather than its nuclear translocation; (iii) PKC thatsignals to promote phosphorylation and degradation of both I $kappa$ B $alpha$ and I $kappa$ B $beta$ in the initial stages of the infection; (iv) ROI generatedby a nonmitochondrial pathway; (v) phosphorylation and proteasomaldegradation of the I $kappa$ B proteins, the former event appearing tobe more important than the latter; and finally (vi) new I $kappa$ B $beta$ ,synthesized in a nonphosphorylated form in the later stages ofinfection. These results are integrated in the signal transductionpathway in Fig. 7. In what follows, we discuss the various detailsand implications of these findings.

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FIG. 7. Postulated model for NF- $kappa$ B activation by RSV. Unidentified RSV gene product(s) "X" intracellularly activates protein kinases such as PKC that may in turn activate other downstream kinases. Raf, members of the MAPK cascade, and ribosomal protein S6 kinase (pp90^rsk) are some postulated examples (see text for details). Inhibition of PP2A by P may lead to a higher steady-state level of the phosphorylated product of any of these kinases; however, it is also possible that the kinases themselves are regulated by PP2A.

Although the recombinant P protein activated RelA, the low levels of activation suggested that there must be other viral geneproducts that play additional or more important roles in an RSV-infectedcell. It remains to be determined whether these entities are RNAor protein in nature and how exactly they interact with the cellularsignal transduction machinery. At least for the P gene of RSV,our evidence suggests that its protein product and not the mRNAis the primary signal, since introduction of premature translationstop codons in the pcDNA3-P clone abolished P protein expressionas well as RelA activation (Fig. 4C). The xanthate compound D609was previously shown to inhibit the growth of at least two nonsegmentednegative-strand RNA viruses, vesicular stomatitis virus (41)and RSV (55). Subsequent studies revealed that it inhibitedthe synthesis of a number of viral proteins, including a 78-foldreduction of the viral N protein and a 7-fold reduction of theP protein. Nonetheless, replication of the RSV genome remainedunaffected (55), which was somewhat surprising, since de novosynthesis of N proteins of negative-strand RNA viruses, includingthose of vesicular stomatitis virus and RSV, is essential forviral RNA replication (reviewed in reference 6). The phosphorylationof the P protein of RSV appeared to be affected by D609 even moredrastically (55). It was therefore hypothesized that D609 inhibiteda viral morphogenetic step, perhaps requiring phosphorylationof the P protein (55). Based on the results presented here,it is possible that any or some of these viral targets of D609may be involved in the function, rather than the nuclear translocation,of RelA. Clearly, identification of the exact viral target(s)of D609 should clarify this issue.

On the other hand, activation of NF- $kappa$ B by a number of cellular agonists, such as TNF, has also been shown to be inhibitedby D609 (47). It was long thought that this is due to the factthat D609 is a direct and specific inhibitor of phosphotidylcholine-specificPLC (1, 16); however, PLD was also shown to be inhibitedrecently (32). Since D609 failed to inhibit the nuclear translocationof RelA (Fig. 3B), neither PLC nor PLD may be required for theinactivation of I $kappa$ B by RSV. In accordance with our results, arecent study has indeed postulated that D609 may inhibit the DNA-bindingactivity of nuclear NF- $kappa$ B by inhibiting a putative accessory factorrequired for NF- $kappa$ B function (16); the identity of the factorand the effect of D609 on it remain to be determined.

It was quite obvious that in the early phase of NF- $kappa$ B activation by RSV, both the I $kappa$ B proteins were destroyed and essentiallydisappeared by 4 to 5 h p.i. (Fig. 3C and D). Both inhibitors,however, reappeared at around 8 h p.i. As has been shown for otherNF- $kappa$ B agonists, this is most certainly due to the transcriptionalinduction of the I $kappa$ B genes by activated NF- $kappa$ B, since all of thedrugs that inhibited NF- $kappa$ B activation also blocked the reappearanceof the I $kappa$ Bs (Fig. 3). In contrast, the newly synthesized I $kappa$ Bsappeared to escape phosphorylation and degradation during thepersistent activation of NF- $kappa$ B by RSV, suggesting that the increasedsynthesis probably overwhelmed the activation signals and thatthe nonphosphorylated form of I $kappa$ B $beta$ may in fact protect RelA frominhibition by I $kappa$ B $alpha$ (44, 54). Two major lines of recent evidencelend precedence to our findings. The first is derived from studiesof the Tax protein of human T-lymphotrophic virus type 1, whichremains the most extensively studied viral activator of NF- $kappa$ Bto date. Tax is known to persistently activated NF- $kappa$ B, and a recentstudy of its mechanism has revealed that expression of the proteinresulted in the degradation of both species of I $kappa$ B, at least atthe early times (40). Interestingly, activation of PKC by Taxwas also shown to be essential for Tax-mediated activation ofNF- $kappa$ B (36). Second, as mentioned earlier, underphosphorylatedI $kappa$ B $beta$ , synthesized during persistent activation of NF- $kappa$ B by TNFor phorbol esters, was shown to form complexes with RelA (p65)that were transcriptionally active and insensitive to I $kappa$ B $beta$ (54).Thus, RSV seems to employ a combination of these two mechanismsto persistently activate RelA. It remains to be seen whether I $kappa$ B $beta$ also reappears in the persistent activation of NF- $kappa$ B by Tax.

The inhibitory effects of a variety of PKC inhibitors strongly implicated a role of PKC enzymes in the activation of RelAby RSV. Chelerythrine A, another specific PKC inhibitor, had similareffects (data not shown). The pseudosubstrate peptide Myr- $psi$ PKCis known to inhibit at least three PKC isozymes: $alpha$ , $beta$ , and $gamma$ .Use of more specific inhibitors and antisense oligonucleotidesagainst specific isozymes should allow us to identify the particularisozyme(s) of PKC that is involved in NF- $kappa$ B activation by RSV.We want to note here that the atypical isozyme PKC- $zeta$ has recentlybeen implicated to play a role in the activation of NF- $kappa$ B by simianvirus (SV40) small t antigen (49) (see below) and by human immunodeficiencyvirus (24).

PDTC is an efficient scavenger of reactive oxygen; thus, its strong inhibitory effect on nuclear translocation of RelA byRSV suggests a major role of ROIs in this pathway. PDTC preventedthe phosphorylation of I $kappa$ B $alpha$ (Fig. 3), indicating that the ROIswork upstream of the phosphorylation step. The inability of rotenoneto inhibit the process suggested that the reactive oxygens areprobably of nonmitochondrial origin. As expected, the specificantiproteasome drug MG132 must act at the distal end of the signalingpathway, since unlike the other drugs, it allowed phosphorylationof both I $kappa$ B polypeptides but prevented the degradation of thephosphorylated end products. Curiously, both I $kappa$ B $alpha$ and I $kappa$ B $beta$ wereaffected in a comparable manner by the inhibitor drugs, suggestingthat the mechanisms of their inactivation as well as resynthesismay share similar, if not identical, features. Similar conclusionshave recently been derived from studies of a mutant cell lineexhibiting a lack of degradation of all kinds of I $kappa$ B proteins(18). In contrast to I $kappa$ B $alpha$ , the mechanism of regulation of I $kappa$ B $beta$ is virtually unknown, although a role of phosphorylation and proteolysisis strongly implicated (30, 57). It was, therefore, concludedthat phosphatases rather than kinases may be the major regulatorsof I $kappa$ B $beta$ phosphorylation. It is tempting to speculate that thephosphatase in question is PP2A and that its inhibition by theRSV P protein may be a major contributor of increased I $kappa$ B $beta$ phosphorylationas observed by us. The stabilizing effect of MG132 on phosphorylatedI $kappa$ B $beta$ is also in agreement with our finding and indicates a roleof proteasomes in I $kappa$ B $beta$ degradation as well (30, 57). It isnoteworthy that none of the inhibitors tested here seemed to inhibitthe early activation of RelA by RSV. Recent studies have indicatedthat at least a part of the early activation is due to the bindingof the virus to its receptors and occurs even in the absence ofviral gene expression (23). This mechanism may, therefore, employmembrane-bound signaling molecules and a signal transduction pathwayfundamentally different from that of persistent activation.

The activation of a signaling pathway through the sequestration and inhibition of a phosphatase by a nonsubstrate phosphoprotein,as suggested by our studies, is without a direct precedent. However,a number of earlier findings provide indirect support for thisnovel mechanism. First, whereas a variety of phosphorylated proteins(such as casein, histone, and lysozyme) are excellent substratesfor all phosphatases, the corresponding thiol-phosphorylated proteinscontaining nonhydrolyzable thiophosphate groups, produced in vitroby using $gamma$ -thio-ATP, are phosphatase resistant, as expected. However,they still retain the capacity to bind phosphatases and have infact been traditionally used to affinity purify phosphatases (28).While a substrate phosphoprotein must also bind the phosphatase,the catalytic role of the enzyme demands that the binding be reversible.In other words, the substrate must dissociate from the enzymefollowing the removal of the phosphate group so that the enzymecan then act on the next substrate molecule. In principle, therefore,a stable and irreversible sequestration of the phosphatase canbe achieved by a nonsubstrate phosphoprotein which would bindto the substrate-binding domain of the phosphatase but not interactwith the enzyme's catalytic domain, perhaps due to the lack ofa proper sequence or conformation around the phosphate groups.We postulate the P protein of RSV satisfies these criteria. Interestingly,the inhibition of PP2A by P protein was not detectable when pNPPwas used as the substrate. While we do not know the exact reasonbehind this, perhaps the simplest scenario that may explain allof these findings is that PP2A contains a substrate-binding domainwhich is distinct from the catalytic site of the enzyme. Bindingof the large P protein to this domain may prevent binding of othermacromolecular substrates by steric hindrance. However, the smallmolecular substrate pNPP may not require the protein substrate-bindingsite and can directly access the catalytic pocket even when Pprotein is bound to the enzyme.

Second, as indicated earlier, potent phosphatase inhibitors, such as OA and calyculin, activate RelA in cells of various origins(30, 52, 53). We have made essentially similar observationswhen using OA (at 3 nM) on A549 cells (data not shown). RSV P,like these toxins, strongly inhibits PP2A (Fig. 5) and thereforemay activate RelA through similar mechanisms. The lack of associationof P with PP1 or PP2B points to the specificity and importanceof the P-PP2A interaction. We predict that the steady-state levelsof a variety of cellular phosphoproteins that are otherwise substratesfor PP2A may also undergo an increase in cells expressing theP protein. As a corollary, RSV infection may affect cellular metabolismin many different ways that are yet uncharacterized. This is currentlybeing tested.

Among the best-studied examples of PP2A regulation are those accomplished by SV40 T antigens and CK2. Detailed studies byWalter and Mumby have shown that the SV40 small t antigen inhibitsPP2A by directly associating with the catalytic subunit C, althoughthe exact amino acid residues involved in the association remainto be identified (reviewed in reference 56). Curiously, thisled to activation of the mitogen-activated protein kinase (MAPK)cascade and NF- $kappa$ B, most likely through the stimulation of theatypical PKC isozyme $zeta$ (49). An intriguing relationship betweena kinase and a phosphatase has been revealed by the recent demonstrationthat the catalytic $alpha$ subunit of CK2 also binds to PP2A in vitroand in mitogen-starved cells and that the overexpression of CK2 $alpha$ resulted in deactivation of the MAPK pathway and suppression ofcell growth (31). These results suggested that PP2A serves animportant role in cell signaling and that its sequestration byCK2 $alpha$ abrogates cell growth. Interestingly, the binding of CK2 $alpha$ to PP2A required the sequence motif HENRKL, common to both CK2 $alpha$ and small t antigen (31). This sequence motif, however, is absentin RSV P protein (39). Thus, RSV P may use a novel sequencemotif to interact with the catalytic subunit of PP2A, or it mayassociate with one of the regulatory subunits of PP2A. A detailedknowledge of which subunits of the PP2A holoenzyme are presentin the RSV P immunoprecipitate will be a starting point in resolvingthe nature of P-PP2A interaction.

It is interesting to us that an essentially cytoplasmic negative-strand RNA virus exploits some of the downstream signalingmolecules that are normally used by physiological agonists toactivate cellular NF- $kappa$ B. The chain of signaling events must betriggered by specific RSV gene products that need to be characterized,although our results suggest that the phosphoprotein P is likelyto be one of them. It will be important to determine whether thecontinued presence of these gene products is needed to maintainthe persistent activation of NF- $kappa$ B. Nevertheless, based on theforegoing, we propose that these gene products activate intracellularPKC, which in turn may signal through a variety of potential kinasesincluding members of the Raf/MAPK pathway (Fig. 7). In additionto human immunodeficiency virus and SV40 as mentioned earlier(24, 49), adenovirus was recently shown to stimulate of theRaf/MAPK signaling pathway, and this was required for the inductionof IL-8 gene expression in adenovirus-infected cells (14). Finally,recent studies suggested that MEKK1, a member of the MAPK cascade,could indeed activate the multisubunit I $kappa$ B $alpha$ kinase complex (35).At least some of the MAPK appeared to activate the ribosomal proteinS6 kinase (pp90^rsk), which could in turn directly phosphorylate I $kappa$ B $alpha$ (27, 37).The role of these kinases in RSV-mediated phosphorylation of I $kappa$ Bproteins is currently under investigation.

	ACKNOWLEDGMENTS

This research was supported in part by a grant-in-aid award (AL G970031) from the American Heart Association (Alabama Affiliate)(to S.B.).

We thank Warren Zimmer (Department of Structural and Cellular Biology) for allowing us to use his luminometer and Sean Dobsonfor sharing unpublished results on D609.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, MSB 2140, College of Medicine, Universityof South Alabama, 307 University Blvd., Mobile, AL 36688-0002.Phone: (334) 460-6860. Fax: (334) 460-6127. E-mail: sbarik{at}jaguar1.usouthal.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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3. Anderson, L. J., and C. A. Heilman. 1995. Protective and disease-enhancing immune responses to respiratory syncytial virus. J. Infect. Dis. 171:1-7[Medline].

4. Ansai, T., L. C. Dupuy, and S. Barik. 1996. Interactions between a minimal protein serine/threonine phosphatase and its phosphopeptide substrate sequence. J. Biol. Chem. 271:24401-24407[Abstract/Free Full Text].

5. Arnold, R., B. Humbert, H. Werchau, H. Gallati, and W. Konig. 1994. Interleukin-8, interleukin-6, and soluble tumour necrosis factor receptor type I release from a human pulmonary epithelial cell line (A549) exposed to respiratory syncytial virus. Immunology 82:126-133[Medline].

6. Banerjee, A., S. Barik, and B. P. De. 1991. Gene expression of nonsegmented negative strand RNA viruses. Pharmacol. Ther. 51:47-70[Medline].

7. Barik, S. 1992. Transcription of human respiratory syncytial virus genome RNA in vitro: requirement of cellular factor(s). J. Virol. 66:6813-6818[Abstract/Free Full Text].

8. Barik, S. 1993. Expression and biochemical properties of a protein serine/threonine phosphatase encoded by bacteriophage $lambda$ . Proc. Natl. Acad. Sci. USA 15:10633-10637.

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1.	Amtmann, E. 1996. The antiviral, antitumoural xanthate D609 is a competitive inhibitor of phosphatidylcholine-specific phospholipase C. Drugs Exp. Clin. Res. 22:287-294[Medline].
2.	Ananaba, G. A., and L. J. Anderson. 1991. Antibody enhancement of respiratory syncytial virus stimulation of leukotriene production by a macrophage-like cell line. J. Virol. 65:5052-5060[Abstract/Free Full Text].
3.	Anderson, L. J., and C. A. Heilman. 1995. Protective and disease-enhancing immune responses to respiratory syncytial virus. J. Infect. Dis. 171:1-7[Medline].
4.	Ansai, T., L. C. Dupuy, and S. Barik. 1996. Interactions between a minimal protein serine/threonine phosphatase and its phosphopeptide substrate sequence. J. Biol. Chem. 271:24401-24407[Abstract/Free Full Text].
5.	Arnold, R., B. Humbert, H. Werchau, H. Gallati, and W. Konig. 1994. Interleukin-8, interleukin-6, and soluble tumour necrosis factor receptor type I release from a human pulmonary epithelial cell line (A549) exposed to respiratory syncytial virus. Immunology 82:126-133[Medline].
6.	Banerjee, A., S. Barik, and B. P. De. 1991. Gene expression of nonsegmented negative strand RNA viruses. Pharmacol. Ther. 51:47-70[Medline].
7.	Barik, S. 1992. Transcription of human respiratory syncytial virus genome RNA in vitro: requirement of cellular factor(s). J. Virol. 66:6813-6818[Abstract/Free Full Text].
8.	Barik, S. 1993. Expression and biochemical properties of a protein serine/threonine phosphatase encoded by bacteriophage $lambda$ . Proc. Natl. Acad. Sci. USA 15:10633-10637.
9.	Barik, S., T. McLean, and L. C. 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].
10.	Baeuerle, P. A., and T. Henkel. 1994. Function and activation of NF- $kappa$ B in the immune system. Annu. Rev. Immunol. 12:141-180[Medline].
11.	Becker, S., H. S. Koren, and D. C. Henke. 1993. Interleukin-8 expression in normal nasal epithelium and its modulation by infection with respiratory syncytial virus and cytokines tumor necrosis factor, interleukin-1, and interleukin-6. Am. J. Respir. Cell Mol. Biol. 8:20-27.
12.	Becker, S., J. Quay, and J. Soukup. 1991. Cytokine (tumor necrosis factor, IL-6, and IL-8) production by respiratory syncytial virus-infected human alveolar macrophages. J. Immunol. 147:4307-4312[Abstract].
13.	Bitko, V., A. Velazquez, L. Yang, Y. C. Yang, and S. Barik. 1997. Transcriptional induction of multiple cytokines by human respiratory syncytial virus requires activation of NF- $kappa$ B and is inhibited by sodium salicylate and aspirin. Virology 232:369-378[Medline].
14.	Bruder, J. T., and I. Kovesdi. 1997. Adenovirus infection stimulates the Raf/MAPK signaling pathway and induces expression of interleukin-8 expression. J. Virol. 71:398-404[Abstract].
15.	Chen, Z., J. Hagler, V. J. Palombella, F. Melandri, D. Scherer, D. Ballard, and T. Maniatis. 1995. Signal-induced site-specific phosphorylation targets I $kappa$ B $alpha$ to the ubiquitin-proteasome pathway. Genes Dev. 9:1586-1597[Abstract/Free Full Text].
16.	Cobb, R. R., K. A. Felts, G. C. Parry, and N. Mackman. 1996. D609, a phosphatidylcholine-specific phospholipase C inhibitor, blocks interleukin-1 $beta$ -induced vascular cell adhesion molecule 1 gene expression in human endothelial cells. Mol. Pharmacol. 49:998-1004[Abstract].
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Persistent Activation of RelA by Respiratory Syncytial Virus Involves Protein Kinase C, Underphosphorylated IB, and Sequestration of Protein Phosphatase 2A by the Viral Phosphoprotein

Persistent Activation of RelA by Respiratory Syncytial Virus Involves Protein Kinase C, Underphosphorylated I $kappa$ B $beta$ , and Sequestration of Protein Phosphatase 2A by the Viral Phosphoprotein