Recombinant Respiratory Syncytial Virus That Does Not Express the NS1 or M2-2 Protein Is Highly Attenuated and Immunogenic in Chimpanzees

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Journal of Virology, October 2000, p. 9317-9321, Vol. 74, No. 19
0022-538X/00/$04.00+0

Recombinant Respiratory Syncytial Virus That Does Not Express the NS1 or M2-2 Protein Is Highly Attenuated and Immunogenic in Chimpanzees

Michael N. Teng,¹ Stephen S. Whitehead,¹ Alison Bermingham,¹ Marisa St. Claire,² William R. Elkins,³ Brian R. Murphy,¹ and Peter L. Collins¹^,^*

Respiratory Viruses Section¹ and Experimental Primate Virology Section,³ Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, Bethesda, Maryland, 20892, and Bioqual, Inc., Rockville, Maryland, 20850²

Received 11 May 2000/Accepted 28 June 2000

	ABSTRACT

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Mutant recombinant respiratory syncytial viruses (RSV) which cannot express the NS1 and M2-2 proteins, designated rA2 $Delta$ NS1and rA2 $Delta$ M2-2, respectively, were evaluated as live-attenuatedRSV vaccines. The rA2 $Delta$ NS1 virus contains a large deletion thatshould have the advantageous property of genetic stability duringreplication in vitro and in vivo. In vitro, rA2 $Delta$ NS1 replicatedapproximately 10-fold less well than wild-type recombinant RSV(rA2), while rA2 $Delta$ M2-2 had delayed growth kinetics but reacheda final titer similar to that of rA2. Each virus was administeredto the respiratory tracts of RSV-seronegative chimpanzees to assessreplication, immunogenicity, and protective efficacy. The rA2 $Delta$ NS1and rA2 $Delta$ M2-2 viruses were 2,200- to 55,000-fold restricted inreplication in the upper and lower respiratory tracts but induceda level of RSV-neutralizing antibody in serum that was only slightlyreduced compared to the level induced by wild-type RSV. The replicationof wild-type RSV in immunized chimpanzees after challenge wasreduced more than 10,000-fold at each site. Importantly, rA2 $Delta$ NS1and rA2 $Delta$ M2-2 were 10-fold more restricted in replication in theupper respiratory tract than was the cpts248/404 virus, a vaccinecandidate that retained mild reactogenicity in the upper respiratorytracts of 1-month-old infants. Thus, either rA2 $Delta$ NS1 or rA2 $Delta$ M2-2might be appropriately attenuated for this age group, which isthe major target population for an RSV vaccine. In addition, theseresults show that neither NS1 nor M2-2 is essential for RSV replicationin vivo, although each is important for efficientreplication.

	TEXT

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Respiratory syncytial virus (RSV) is the leading etiologic agent of serious pediatric viral bronchiolitis and pneumonia worldwideand is responsible for approximately 100,000 hospitalizationsand 4,500 deaths among infants and children in the United Statesper annum (7, 14, 25). In addition, RSV infection can causesevere respiratory illness in the elderly (23) and in immunocompromisedindividuals (28). To date, an effective licensed vaccine forRSV is not available despite the pressing need for such anagent.

Since 1967, our laboratory has focused on developing a live-attenuated RSV vaccine for intranasal administration. By mimickinga natural infection, such a vaccine should stimulate both cellularand humoral immunity and would obviate the potentiated diseasethat was observed with certain nonreplicating or subunit vaccines(7, 16, 24, 27). The intranasal route also partiallyabrogates the immunosuppressive effects of maternal antibodiespresent in the sera of young infants and stimulates both localand systemic immunity (10).

A number of live-attenuated RSV vaccine candidates have been developed by biological or recombinant methods and evaluatedin animals and humans (8, 15, 16, 29, 30, 32). Themost promising biologically derived candidate, a cold-passaged(cp) temperature-sensitive (ts) virus called cpts248/404, wasevaluated in RSV-naive 1- to 2-month-old infants and was foundto be infectious, immunogenic, and protective against a secondvaccine dose (33). However, some vaccinees experienced mildupper respiratory tract congestion, indicating that further attenuationis necessary. In addition, virus isolated late during the courseof infection from a single vaccinee showed partial phenotypicreversion and loss of an attenuating mutation. Thus, our strategyto develop improved live-attenuated vaccine candidates has been(i) to use recombinant methods to combine attenuating mutationsidentified in a panel of biologically derived attenuated virusesincluding cpts248/404 and (ii) to develop new types of attenuatingmutations by focusing on gene deletions which should be refractoryto geneticreversion.

RSV is the prototype member of the Pneumovirus genus of the family Paramyxoviridae. Its genome is a single-stranded, negative-senseRNA of 15.2 kb that encodes 10 subgenomic mRNAs from which 11proteins are translated. These proteins include the nucleocapsidN protein, phosphoprotein P, and large polymerase subunit L, whichtogether comprise the minimal viral polymerase; fully processivetranscription by the RSV polymerase requires the presence of thetranscription antitermination factor M2-1 (6, 18, 19, 34).There are four envelope-associated proteins: the internal matrix(M) protein and three transmembrane surface proteins, namely,the attachment (G), fusion (F), and small hydrophobic (SH) proteins(7). Finally, RSV encodes two nonstructural proteins, NS1 andNS2, and also the M2-2 protein, whose status as structural ornonstructural is unknown. NS1 and M2-2 appear to have roles inRNAsynthesis.

We previously described a reverse-genetics system for producing recombinant subgroup A RSV (rRSV) by coexpression of antigenomicRNA and the N, P, L, and M2-1 proteins from cotransfected plasmids(5). One application of this system has been to identify viralgenes that can be deleted or silenced without ablating replicationin vitro but are still necessary for virus replication in vivo(4, 26). Deletion of the SH gene resulted in a virus, designatedrA2 $Delta$ SH, that replicated in vitro with an efficiency equal to orslightly better than that of wild-type rRSV (rA2) and which wasmoderately attenuated in mice and chimpanzees (4, 29). rRSVfrom which the NS2 gene was deleted, designated rA2 $Delta$ NS2, exhibitedreduced growth kinetics and a reduced yield of infectious virusin vitro and was markedly attenuated in mice and chimpanzees (26,29). Similar in vitro properties were noted for a recombinantbovine RSV from which the NS2 gene was deleted (2). These twodeletion mutations are now being incorporated into recombinantlive-attenuated vaccine candidates for clinicalevaluation.

More recently, the M2-2 open reading frame was silenced in rRSV (rA2 $Delta$ M2-2, previously designated rA2-K5) by mutating eachof the three potential translational initiation codons and insertinga translation termination codon in each of the three reading frames(1). A second research group made a comparable virus in whichM2-2 was silenced by deletion of most of its open reading frame,which resulted in a virus that appeared to be phenotypically similarto rA2 $Delta$ M2-2 (20). The rA2 $Delta$ M2-2 virus exhibited increased plaquesize, reduced growth kinetics (though the final titer was similarto that of the wild type), and a partial shift in RNA synthesisfrom RNA replication to transcription (1). Thus, the M2-2 proteinappears to be a regulatory protein that negatively regulates transcriptionand positively regulates RNA replication. In addition, an rRSVwas constructed from which the NS1 gene was deleted by the removalof nucleotides 122 to 630 in the antigenomic cDNA, resulting inthe joining of the upstream nontranslated region of NS1 to thetranslational initiation codon of NS2. This virus, designatedrA2 $Delta$ NS1, exhibited reduced RNA replication, plaque size, and growthkinetics and an approximately 10-fold lower yield of infectiousvirus in vitro (M. N. Teng and P. L. Collins, submitted for publication).Other paramyxoviruses encode proteins, such as the V protein ofSendai virus, that are not essential for replication in vitro.However, ablation of expression of V by recombinant Sendai virusresults in attenuation in vivo (22). It was suggested that thisprotein functioned to antagonize some aspect of the mouse's innateimmune system. More recently, the V protein of simian virus 5was shown to block signalling for both type I and type II interferonresponses (13). Any of the RSV "accessory" proteins, includingthe NS1, NS2, M2-2, SH, and G proteins, are candidates for antagonizinghost immunemechanisms.

In the present study, we evaluated the rA2 $Delta$ M2-2 and rA2 $Delta$ NS1 viruses for replication, immunogenicity, and protective efficacyin the upper and lower respiratory tracts of chimpanzees, theonly experimental animal in which RSV replication and virulenceapproaches that observed in humans. The rA2 $Delta$ M2-2 and rA2 $Delta$ NS1 virusesdescribed above were constructed in the original version of theantigenomic cDNA described by Collins et al. (5). All recombinantviruses that have been constructed for vaccine purposes in ourlaboratory contain two types of modification to this background:(i) the introduction of a set of six translationally silent restrictionmarkers in the L gene, called the sites mutations, and (ii) twoamino acid substitutions in the F protein, called the HEK mutations,which make the recombinant virus identical at the amino acid levelto the wild-type RSV A2 parent from which the cpts248/404 seriesof biological vaccine candidates was derived (21, 30). Thesemutations were shown to be phenotypically silent in chimpanzees(32). The rA2 $Delta$ NS1 virus used in this study was reconstructedin a sites-HEK background, in preparation for clinical evaluation,whereas the rA2 $Delta$ M2-2 virus is in the original genetic background,a difference that is not relevant for the present study (1,30).

The rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 viruses were administered individually to juvenile RSV-seronegative chimpanzees by combined intranasaland intratracheal inoculation, as described previously (11).Since both viruses were attenuated in vitro, we chose to inoculatethe animals with 10⁵ PFU per ml per site, which is a 10-fold higher concentrationthan that typically used to inoculate chimpanzees. To monitorvirus replication in the upper and lower respiratory tracts, respectively,nasopharyngeal swabs and tracheal lavage samples were collectedat intervals over 10 days postinfection and subsequently wereassayed for virus titer. The mean peak virus titer was determinedfor each group (Table 1). The chimpanzees were monitored dailyfor rhinorrhea, a symptom of upper respiratory tract illness,and the mean peak score was determined for each group (Table 1).Due to the limited availability of RSV-seronegative chimpanzees,the number of animals per group was small, making it necessaryto include controls from previous studies in which we had evaluatedbiologically derived RSV strain A2 (wild-type RSV A2), rA2, rA2 $Delta$ SH,rA2 $Delta$ NS2, and a recombinant version of the above-mentioned cpts248/404vaccine candidate (rA2cp248/404) (Table 1).

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TABLE 1. rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 are highly attenuated in both the upper and lower respiratory tracts of chimpanzees but are highly immunogenic

Levels of replication of rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 were reduced more than 2,200-fold and more than 2,800-fold, respectively, inthe upper respiratory tract compared to that of rA2 (Table 1).Shedding of rA2 $Delta$ NS1 or rA2 $Delta$ M2-2 was detected sporadically andat a low level beginning 2 to 7 days postinfection, and each animalshed virus over a period of 3 to 8 days (data not shown). Thus,the recovered virus was not carried over from the initial inoculumbut represented replication near the level of detection over aperiod of several days. In the lower respiratory tract, the levelof replication of rA2 $Delta$ NS1 was reduced more than 17,000-fold comparedto that of rA2, while rA2 $Delta$ M2-2 was undetectable at all time points(greater than 55,000-fold reduction). It is important to notethat the dose of rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 used was 10-fold greaterthan that of rA2. Furthermore, both viruses were more attenuatedthan rA2cp248/404, which was given at the same dose, particularlyin the case of rA2 $Delta$ M2-2, which was not recovered from the lungsof infected chimps. In addition, both rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 wereunusual in being equally restricted in the upper and lower respiratorytracts. In the upper respiratory tract, each virus was approximately10-fold more restricted than cpts248/404 and 175-fold more restrictedthan rA2 $Delta$ NS2. Since upper respiratory tract congestion was observedduring clinical evaluation of the cpts248/404 virus in 1- to 2-month-oldinfants (33) and since infants of that age are obligate nosebreathers, mutations that confer a level of restriction of replicationin the upper respiratory tract greater than that of cpts248/404would be desirable for inclusion in a live-attenuated vaccinevirus. Animals receiving rA2 $Delta$ NS1 or rA2 $Delta$ M2-2 had slightly morerhinorrhea than those infected with rA2cp248/404, though stillless than that of animals infected with a 10-fold smaller doseof rA2. While it is possible that the absence of NS1 or M2-2 resultedin a virus that retained a moderate level of virulence but replicatedpoorly, we think that this possibility is unlikely. Our experienceis that quantitation of rhinorrhea and the comparison of suchvalues from different studies performed at different times canbe somewhat subjective and hence not completely reproducible.We anticipate that further evaluation, including clinical studies,will show that the amount of residual virulence associated withrA2 $Delta$ NS1 and rA2 $Delta$ M2-2 will reflect their greatly reducedreplication.

Despite the highly restricted replication of these viruses, immunization with either rA2 $Delta$ NS1 or rA2 $Delta$ M2-2 induced a level ofRSV-neutralizing antibody in serum that was within threefold ofthat induced by rA2cp248/404 (Table 1). Furthermore, animalspreviously infected with either rA2 $Delta$ NS1 or rA2 $Delta$ M2-2 were highlyresistant to the replication of wild-type RSV administered intranasallyand intratracheally 56 days postimmunization (Table 2). The levelsof protection in both cases were similar in the upper respiratorytract and somewhat lower in the lower respiratory tract than thatseen with cpts248/404, both in mean peak titer and in mean daysof shedding.

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TABLE 2. Infection of chimpanzees with rA2 $Delta$ NS1 or rA2 $Delta$ M2-2 induced significant protection against subsequent challenge with wild-type RSV A2 in the upper and lower respiratory tracts

The challenge in developing a live-attenuated RSV vaccine is to eliminate residual virulence without compromising immunogenicity.Observations to date indicate that the severity of RSV diseaseis closely related to the level of RSV replication in the respiratorytract. It is possible that one or more attenuating mutations thatreduce virulence through another mechanism will be identified;indeed, it was hoped that deletion of one or more of the nonessentialRSV proteins, such as those described in the present paper, mightreveal such a virulence factor. However, a factor of this naturehas not yet been identified for RSV. Thus, the present methodfor attenuating RSV is to reduce its level of replication, whichunfortunately can reduce its immunogenicity due to the reducedproduction of antigen. The attenuating mutations that we haveidentified to date include (i) a set of five amino acid substitutionsin the N, F, and L proteins that were identified in cpRSV andthat confer attenuation in chimpanzees and humans (9, 16,32); (ii) a series of amino acid substitutions in the L proteinand a nucleotide substitution in the gene-start signal of theM2 gene, which were identified in biologically derived ts derivativesof cp RSV and which each confer the ts and attenuation phenotypes(12, 15, 21, 30); and (iii) deletion of individual orcombinations of RSV genes such as the SH and NS2 genes (4,26). Bovine RSV genes have also been used to confer attenuationbased on host range restriction (3). Here, we add two additionalknockout mutations to the list, namely, the deletion of NS1 andthe silencing of the M2-2 open readingframe.

Among the mutant viruses shown in Table 1, the order of increasing attenuation in seronegative juvenile chimpanzees was rA2 $Delta$ SH< rA2 $Delta$ NS2 < rA2cp248/404 < rA2 $Delta$ NS1 < rA2 $Delta$ M2-2. All viruses providedsimilar, high levels of protection against challenge with wild-typeRSV (Table 2). Thus, rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 each have the desiredproperty of being slightly more attenuated than rA2cp248/404,the recombinant version of cpts248/404, which was slightly tooreactogenic in RSV-naive 1- to 2-month-old infants, as mentionedabove (33). The finding that rA2 $Delta$ M2-2 is slightly more attenuatedthan rA2 $Delta$ NS1 increases the chances that one of these viruses willhave an optimal level of attenuation. The seronegative juvenilechimpanzee is somewhat less permissive to RSV replication anddisease than is the RSV-naive human infant. Thus, whether rA2 $Delta$ NS1,rA2 $Delta$ M2-2, or both have an appropriate level of attenuation canbe determined only by clinical trials with the target vaccinepopulation, 1- to 2-month-oldinfants.

Deletion mutants should be extremely stable both in vitro and in vivo, thus making them attractive candidates for vaccinedevelopment. This property might be important in light of thefinding that one infant who had been vaccinated with cpts248/404shed virus that exhibited a partial reversion (33). A low levelof genetic instability in an RSV vaccine likely would not be aproblem in normal individuals, particularly considering the highprevalence of fully virulent wild-type RSV. However, vaccine virusmight have prolonged replication in immunocompromised individuals.Thus, it would be desirable to engineer a recombinant vaccinevirus to contain attenuating mutations that cannotrevert.

Although the major target for an RSV vaccine is the 1- to 2-month-old infant, a second target is the elderly. The cpts248/404vaccine candidate, which was insufficiently attenuated in theRSV-naive infant, was found to be overattenuated in the RSV-experiencedadult (17). Thus, a live-attenuated vaccine for RSV-naive infantswill need to be more attenuated than one for use in adults. Sincethe rA2 $Delta$ NS1 and rA2 $Delta$ M2-2 viruses are similar to cpts248/404 intheir levels of replication, they likely will be too attenuatedto be useful as an adult vaccine. However, each virus is appropriatefor further evaluation as a pediatric RSV vaccine, either as currentlyconstructed or with the inclusion of a single or a combinationof additional attenuating mutations. It should be noted that ifeither candidate vaccine proves satisfactory, a partner subgroupB candidate can be rapidly generated by replacing the F and Gglycoproteins (31).

	ACKNOWLEDGMENTS

We thank Robert Chanock for criticalreview.

This work is part of a continuing program of research and development with Wyeth Lederle Vaccines through CRADA no. AI-000087and AI-000099.

	FOOTNOTES

^* Corresponding author. Mailing address: LID, NIAID, 7 Center Dr., MSC 0720, Bethesda, MD 20892-0720. Phone: (301) 496-4205.Fax: (301) 496-8312. E-mail: pcollins{at}niaid.nih.gov.

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Journal of Virology, October 2000, p. 9317-9321, Vol. 74, No. 19
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