Production of Protective Human Antipneumococcal Antibodies by Transgenic Mice with Human Immunoglobulin Loci

doi:10.1128/IAI.68.4.1820-1826.2000

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Infection and Immunity, April 2000, p. 1820-1826, Vol. 68, No. 4
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Production of Protective Human Antipneumococcal Antibodies by Transgenic Mice with Human Immunoglobulin Loci

Nina D. Russell,¹ Jose R. F. Corvalan,² Michael L. Gallo,² C. Geoffrey Davis,² and Liise-anne Pirofski³^,¹^,³^,^*

Department of Medicine, Division of Infectious Disease,¹ and Department of Microbiology and Immunology,³ Albert Einstein College of Medicine, Bronx, New York 10461, and Abgenix, Inc., Fremont, California 94555²

Received 28 September 1999/Returned for modification 15 November 1999/Accepted 3 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Infections with Streptococcus pneumoniae remain a significant cause of morbidity and mortality. To gain insight into structure-functionrelationships for human antibodies to pneumococcal capsular polysaccharide(PPS), we studied the response of transgenic mice reconstitutedwith human immunoglobulin loci, XenoMouse, to PPS antigens ina pneumococcal vaccine. Enzyme-linked immunosorbent assays ofsera from mice vaccinated with a 23-valent pneumococcal vaccinerevealed that they produced serotype-specific human antibodies,with the greatest response being to the PPS of serotype 3 (PPS3). Molecular sequence analysis of three monoclonal antibodies(MAbs) to PPS 3 generated from lymphoid cells from mice vaccinatedwith a 23-valent pneumococcal vaccine or a PPS 3-bovine serumalbumin conjugate revealed that they all used heavy-chain immunoglobulingenes from the V_H3 family, two expressed light chain genes fromthe human V $kappa$ 1 family, and one expressed a mouse $lambda$ light chain.The protective efficacy of the two MAbs was examined in mice.A 10-µg dose of both, and a 1-µg dose of one, significantly prolongedsurvival from a lethal serotype 3 infection in CBA/N mice. Ourdata show that XenoMouse mice produced protective, serotype-specifichuman antibodies to PPS 3, and they lend support to the proposalthat these animals represent a useful model to study the humanantibody response to PPSantigens.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Available pneumococcal vaccines consist of the purified capsular polysaccharides (PPS) of the most common serotypes of Streptococcuspneumoniae that cause disease in adults and children. Though immunogenicin normal individuals, PPS-based vaccines are poorly immunogenicin adult patients who are at increased risk for pneumococcal infections(reviewed in reference 33). Our group and others have shownthat human antibodies to PPS are derived from restricted B-cellsubsets which express V_H3 gene family segments (3, 27, 40).However, these studies were based largely on studies of polyclonalserum antibodies. Characterization of the molecular genetic structureof antibodies to the capsular polysaccharide of Haemophilus influenzaetype b (4, 28) has provided insight into possible mechanismsof disease susceptibility and vaccine failure in patients withdecreased expression of the genetic elements used in the response(16). This is relevant to S. pneumoniae, because overall (8)and serotype-specific V_H3 expression is decreased in human immunodeficiencyvirus-infected individuals (3), a group with reduced responsesto pneumococcal vaccines (reviewed in reference 33) and increasedsusceptibility to pneumococcal infection (23).

To date, the genetic makeup of a limited number of human monoclonal antibodies (MAbs) to a limited number of PPS serotypesgenerated by Epstein-Barr virus transformation of lymphocytesfrom vaccinated recipients has been described, namely, two MAbsto PPS 3 derived from different individuals (39), one to PPS8 (46) and one to PPS 6B (40). Epstein-Barr virus transformationis difficult and unpredictable. In addition, all approaches toproducing MAbs from vaccinated humans are hampered because theimmune response cannot be manipulated experimentally. The developmentof a transgenic mouse strain reconstituted with human immunoglobulinloci, XenoMouse, has made it possible to generate fully humanantibodies in mice (29). XenoMouse animals were created by introducingyeast artificial chromosomes (YACs) containing 66 human heavy-chainand 32 $kappa$ light-chain immunoglobulin genes into mice whose endogenousheavy-chain and $kappa$ loci were functionally inactivated by targeteddeletion (29). The mice express human µ, $delta$ , $gamma$ 2, and $kappa$ chainsand mouse $lambda$ chains, with a human $kappa$ -to-mouse $lambda$ ratio of 75:1 (29).XenoMouse animals were previously shown to produce human antibodiesto protein antigens (19, 29), but their ability to respondto T-independent antigens such as polysaccharides was unknown.This study was undertaken to investigate whether XenoMouse animalsrepresent a useful model to investigate the human antibody repertoiretoPPS.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

S. pneumoniae and PPS. S. pneumoniae serotype 3, strain 10813 (American Type Culture Collection [ATCC], Manassas, Va.), was used for mouse protectionexperiments. Organisms were prepared for animal inoculation asdescribed previously (1) and stored at $-$ 80°C until use. A 23-valentpneumococcal vaccine (Pneumovax 23; Merck & Co., Inc., West Point,Pa.) was used for vaccinations and to coat enzyme-linked immunosorbentassay (ELISA) plates. Purified PPS from S. pneumoniae serotypes3, 4, 6B, 8, and 19F (ATCC) were used for ELISAs. A PPS 3-bovineserum albumin (BSA) conjugate was produced with the purified PPSfrom serotype 3 (ATCC) and BSA (Sigma Chemical Co., St. Louis,Mo.) as described elsewhere (26).

XenoMouse animals and vaccination protocols. Two genetically distinct groups of XenoMouse animals were used: Xm2a-3, reconstituted with one double YAC containing bothheavy- and light-chain genes; and Xm2a-5, reconstituted with twoYACs, one with heavy-chain and the other with light-chain genes(22). All mice were bred and maintained at Abgenix (Fremont,Calif.). Overall, 40 XenoMouse animals (37 female and 3 male)were vaccinated with 11.5 µg of a 23-valent pneumococcal vaccine(consisting of 0.5 µg of each of the 23 PPS antigens in the vaccine)either without (group A [5 animals]) or with (groups B [5 animals]and C and D [15 animals each]) 25 µg of the adjuvant monophosphoryllipid A (Sigma) as described elsewhere (18). The vaccinationswere administered either intraperitoneally (groups A, B, and C)or subcutaneously at the base of the tail (group D). In addition,a group of 10 Xm2a-3 mice was vaccinated at the base of the tailwith 10 µg of the PPS 3-BSA conjugate (see above) without adjuvanton days 1, 15, and 18. The PPS 3-BSA conjugate was used becausethe Pneumovax-vaccinated mice had the greatest serum antibodyresponses to PPS 3 (seebelow).

Serologic studies of antibody responses. Sera were separated by centrifugation from blood obtained from the retro-orbital sinus plexus of the mice and stored at $-$ 20°Cuntil analyzed. The sera were adsorbed with purified pneumococcalcell wall polysaccharide (CWPS; Statens Seruminstitut, Copenhagen,Denmark), and an antigen capture ELISA was used to detect antibodiesto PPS as described elsewhere (3). Briefly, polystyrene ELISAplates (Corning Glass Works, Corning, N.Y.) were coated with eitherPVX (10 µg/ml) or PPS 3, 4, 6B, 8, or 19F (10 µg/ml), blockedwith PBS-1% BSA, washed, and incubated at 37°C for 1 h with a1:50 dilution of the serum samples. After washing, the plateswere incubated at 37°C for 1 h with alkaline phosphatase (AP)-conjugatedgoat antibodies to human immunoglobulin G (IgG), IgM, and kappalight chains and to mouse lambda light chains (Fisher Biotech,Fisher Scientific, Pittsburgh, Pa.) and were then washed. Antibodybinding was detected with p-nitrophenyl phosphate substrate (Sigma)in diethanolamine buffer (pH 9.8). Optical densities (ODs) weremeasured at 405 nm with an MRX microplate reader (Dynatech Laboratories,Chantilly, Va.). Serum from a human PVX recipient which was takenon day 28 postvaccination used at a 1:50 dilution was the positivecontrol on each plate (3). Antibody levels were defined asthe average OD of duplicate wells of the samples minus two timesthe background. The background for each plate was defined as theOD of the detection antibodyalone.

Generation and molecular characterization of hybridomas. Hybridomas were generated by fusion of splenic and/or lymph node cells from XenoMouse animals with the nonsecreting myelomacell line NSO-bcl 2 as described elsewhere (29). The cells usedfor the fusions were from mice vaccinated with the PPS 3-BSA ondays 1, 15, and 18 before fusion on day 21 or from mice that hadreceived PVX vaccinations on days 1, 26, 40, 56, 82, and 87 beforefusion on day 90. The latter vaccination protocol had been usedpreviously for immunization of XenoMouse animals with other antigens.Supernatants from hypoxanthine-aminopterin-thymidine-selectedhybridomas were screened for the production of human antibodiesto PPS by ELISA as described above. Nucleic acid sequencing ofhybridoma heavy (V_H) and light (V_L) chains was performed on PCR-amplifiedV_H and V_L cDNAs as described elsewhere (29, 34). PCR productscorresponding to the human IgM V_H and V $kappa$ were isolated from Tris-acetate-EDTAagarose gels by centrifugation through Spin X columns (FisherBiotech), and both strands of the gel-purified product were directlysequenced as described previously (19). Sequence analysis wasperformed using the Vbase database for sequence alignment andidentification (I. M. Tomlinson et al., MRC Centre for ProteinEngineering) (21). D regions were assigned according to Corbettet al. (12).

Specificity studies of the MAbs. The serotype specificity of the MAbs was determined by ELISA using plates coated with PPS 3, 4, 6B, 8 and 19F as describedabove. The PPS 3 binding of the MAbs was examined by inhibitionELISA after adsorption of the MAbs with 50 µg of CWPS per ml.PPS 3-coated ELISA plates were incubated with the MAbs (5 µg/ml)and concentrations of PPS 3 from 0.01 to 100 µg/ml at 37°C for1 h. The plates were then washed and incubated with AP-conjugatedgoat antibody to human IgM and developed as described above. Cross-reactivityof the MAbs with tetanus toxoid (TT; Connaught, Inc., Swiftwater,Pa.), human IgG Fc (Calbiochem, San Francisco, Calif.), humanDNA (Sigma), and CWPS was examined by ELISA as described elsewhere(34). Briefly, serial dilutions of the MAbs starting at a concentrationof 5 µg/ml (except for MAb 1.4, which was available only at aconcentration of 1 µg/ml) were incubated with antigen-coated plates.A human MAb with reactivity with DNA, TT, and IgG Fc (providedby Anne Davidson, Albert Einstein College of Medicine) was usedas a positive control. The human IgM MAb to PPS 8, D11, was usedas a negative control (46). The MAbs were purified by columnchromatography from ascites (MAbs 1.2, 1.10, and 1.1) or hybridomasupernatants (MAb 1.4).

MAb-mediated complement activation. ELISAs were performed as described elsewhere (46) to determine if the MAbs to PPS 3 could deposit complement component 3(C3) on PPS 3. ELISA plates coated with 10 µg of PPS 3 per mlwere incubated at 37°C for 1 h with solutions containing a finalMAb concentration of 1 or 10 µg/ml and 10% of each complementsource. Factor B-deficient human serum (Calbiochem), which hasan inactive alternative complement pathway, was used to evaluatethe influence of the classical pathway as described elsewhere(46, 47). Normal human serum, adsorbed with PPS 3, beforeand after chelation with 10 mM EGTA (Sigma) and 10 mM MgCl₂, wasused to examine the influence of the alternative pathway as describedelsewhere (17). A myeloma IgM MAb (Calbiochem) was used as anegative control (46, 47). After incubation, the plates werewashed, incubated at 37°C for 1 h with goat anti-human C3 (Sigma),washed, incubated at 37°C for 1 h with AP-conjugated rabbit antibodyto goat IgG (Sigma), and the developed and read as described above.C3 deposition was characterized by OD after subtraction of thebackground due to the complement sources alone. The C3 depositionexperiment was performedtwice.

Mouse protection experiments. Protection studies were performed with MAbs 1.10 and 1.2. The design of the experiments was based on our group's and others'studies of S. pneumoniae infections in mice (9, 10). FemaleCBA/N mice (6 to 8 weeks of age) were obtained from the NationalCancer Institute, Bethesda, Md., and maintained in the AlbertEinstein College of Medicine animal facility prior to use. Mouseinoculations were performed as follows: groups of 10 mice eachreceived 0.5 ml (1 or 10 µg in sterile saline) of MAb 1.2, MAb1.10, the human myeloma IgM control (Calbiochem) used as an isotypecontrol as described elsewhere (46), or PBS intraperitoneally;1 h later, 0.2 ml (300 CFU in tryptic soy broth) of S. pneumoniae(ATCC strain 10813) was given via intravenous inoculation intothe lateral tail vein. The number of CFU injected was confirmedby plating each inoculum that was injected into the mice. Theinoculum was based on the known susceptibility of CBA/N mice toinfection with strain 10813 as described previously (9, 10)and was >100 times greater than the 90% lethal dose for CBA/Nmice determined in our laboratory (data not shown). Mice wereobserved daily. The number of surviving mice in each group wascompared with the Kaplan-Meier log-rank survival test using thestatistical software package SPSS (SPSS, Inc., Chicago, Ill.).The protection experiments were performed twotimes.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Antibody responses to pneumococcal vaccination. The XenoMouse animals in all four vaccination groups produced human IgM and IgG to the PPS antigens in the vaccine. The magnitudeof the IgM response for each group was greater than the IgG response,and there was no significant difference in the response of thefour groups. The binding of preimmune sera to PVX and individualPPS antigens was equal to or less than background (not shown).Five mice were found to have mouse $lambda$ antibodies to the PPS inthe vaccine 1 of 5 from group A, 1 of 5 from group B, 2 of 15from group C, and 1 of 15 from group D. IgM and IgG reactive withPPS 3, 4, 6B, 8, and 19F is shown for a subset of 19 mice withthe highest levels of antibodies to the PPS in the whole vaccine(Fig. 1). Overall, 17 of 19 mice had levels of IgM to PPS 3 thatwere greater than or equal to the level of a human vaccinee. Vaccinationof Xm2a-3 XenoMouse animals with the PPS 3-BSA conjugate elicitedIgM to PPS 3 in 10 of 10 Xm2a-3 mice, but only 3 mice producedIgG to PPS 3 (Fig. 1). The PPS 3 binding of sera from the PPS3-BSA-vaccinated mice was inhibited by soluble PPS 3 (not shown).

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FIG. 1. Serotype-specific responses to the PPS 3, 4, 6B, 8, and 19F in Pneumovax-vaccinated mice. The PPS 3 responses of the PPS 3-BSA-vaccinated mice are shown in the top right panel. The y axes represent the ODs of serum samples from the individual mice depicted on the x axes. 007 and 009 series mice are from groups A and B; all other mice are from groups C and D. The y-axis scales differ for each serotype. For groups A and B, samples tested were from day 47 after vaccinations on days 1, 26, and 40. For groups C and D, samples tested were from day 21 after vaccinations on days 1 and 14. The sera from the PPS 3-BSA-vaccinated mice were from day 18 after vaccinations on days 1 and 15. The sera were used at a dilution of 1:50. The ODs shown represent the values after subtracting two times the background. A day 28 postvaccination serum from a human vaccinee was used as a positive control on each plate at a dilution of 1:50. It had the following serotype-specific ODs: PPS 3, 0.83 (IgM) and 2.15 (IgG; PPS 4, 0.90 and 2.11; PPS 6B, 0.58 and 1.89; PPS 8, 1.42 and 2.09; PPS 19, 1.16 and 2.15. Black bars represent IgM, and cross-hatched bars represent IgG.

Specificity of MAbs. MAbs 1.10, 1.2, and 1.4 reacted with PPS 3, without significant binding (less than or equal to background) to the PPS of serotypes4, 6B, 8, 14, and 19F. Fifty percent of the binding of MAbs 1.10and 1.2 (each at 5 µg/ml) to PPS 3 was inhibited by soluble PPS3 at 0.8 and 2 to 7 µg/ml, respectively; 46% of the binding ofa culture supernatant of MAb 1.4 (0.45 µg/ml) was inhibited bysoluble PPS 3 at 1 µg/ml (not shown). Soluble PPS 3 did not inhibitthe PPS 3 binding of MAbs 1.1 and 2.1 (data not shown), whichwas interpreted to indicate that their PPS 3 binding was nonspecific.The MAbs did not bind to CWPS, DNA, TT, or human IgG Fc (not shown).Hence, the MAbs were not polyreactive and had different avidityfor PPS3.

MAb-mediated complement activation. Since antibody is required for most pneumococcal serotypes, including serotype 3, to active complement (43), the abilityof the PPS 3-specific MAbs 1.2 and 1.10 to deposit C3 on solid-phasePPS 3 was studied. More studies with MAb 1.4 were precluded bythe loss of the cell line. In the presence of EGTA-treated anduntreated human serum, the magnitude of C3 deposition on solid-phasePPS 3 was greater with MAb 1.2 than MAb 1.10 for both MAb concentrations(Fig. 2A). Similarly, in the presence of factor B-deficient serum,the magnitude of C3 deposition was greatest for MAb 1.2, and therewas greater deposition at the higher concentration (Fig. 2B).These results demonstrate that MAb-mediated C3 deposition on PPS3 was greater via the classical than the alternative complementpathway and that MAb 1.2 mediated more complement deposition.The experiments were repeated two times with similar results.

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FIG. 2. MAb-mediated C3 deposition on PPS 3 via activation of the alternative or classical complement pathway. The y axes depict the OD representing C3 deposited on solid-phase PPS 3 in the presence of the MAbs depicted on the x axis, along with the influence of the alternative complement pathway activation in the presence of human sera before and after chelation with EGTA and MgCl₂ (A) and the influence of the classical pathway in the presence of factor B-deficient human serum (B). Each bar represents the average of duplicate wells. For the control IgM in both experiments, C3 binding was detected at ODs of $<=$ 0.1 after subtraction of the background; hence no bars are depicted. Symbols in panel A represent the MAbs at 10 µg/ml in the presence of normal human serum (solid black bars) and in the presence of serum chelated with EGTA and MgCl₂ (hatched black bars) and at 1 µg/ml in the presence of normal human serum (white bars) and in the presence of chelated serum (hatched white bars). In panel B, gray bars represent MAbs at 10 µg/ml, while hatched gray bars represent mAbs at 1 µg/ml; all are in the presence of factor B-deficient serum. The experiments were performed twice, and the results of one experiment are shown.

Genetic makeup of XenoMouse-derived MAbs. The immunoglobulin gene segments used by the three PPS 3-specific MAbs are shown in Table 1. MAb 1.10 was a chimeric antibodythat expressed a human µ and mouse $lambda$ transcript, but it had ahuman $kappa$ transcript with an 18-bp deletion in its J $kappa$ 2 sequencewhich prevented its expression. All the other MAbs expressed bothhuman µ and $kappa$ transcripts without deletions. Each MAb had a differentheavy-chain gene element, each from the V_H3 family: MAb 1.10 usedthe DP-38/9.1/V3-15 gene, MAb 1.2 used the DP 77/V3-21 gene, andMAb 1.4 used the DP 50/V3-33 gene (Table 1). Each MAb had a uniqueV_H CDR 3. Table 2 shows the CDR 3 sequences of the PPS 3-specificXenoMouse-derived MAbs compared to the human MAbs to PPS 3 reportedby Shaw et al. (39) and the nonspecific MAbs produced from thevaccinated XenoMouse mice. The D regions of MAbs 1.10, 1.2, and1.4 use reading frame 1, and those of the nonspecific MAbs usereading frame 2. All of the D regions encode a number of polarand hydrophilic amino acids: glutamine (Q), glycine (G), serine(S), asparagine (N), tyrosine (Y), and threonine (T). The PPS3-specific XenoMouse-derived MAbs all used J_H4 gene segments,whereas the nonspecific MAbs use different J_H genes. All PPS 3-specificMAbs had germ line V_H and V $kappa$ sequences, but the nonspecific MAb1.1 had 3 silent base changes in codons 69, 88, and 93 of theV_H. Taken together, the sequence information revealed that allof the MAbs used genes from the V_H3 family, but the junctionaldiversity of the MAbs indicated that each was the product of adistinct recombination event.

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TABLE 1. Heavy- and light-chain variable gene use of PPS 3-specific MAbs

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TABLE 2. Heavy- and light-chain CDR3 sequences of PPS 3-specific and nonspecific MAbs

Mouse protection experiments. Treatment with MAb 1.2 prolonged the survival of mice infected with serotype 3 S. pneumoniae at both 1- and 10-µg doses, whereasMAb 1.10 prolonged survival at the 10-µg dose only (Fig. 3). Atthe 10-µg dose, mean survival was 1 day for the PBS group, 1 dayfor the control IgM group, 7.8 ± 2.3 days for the MAb 1.10 group,and 17.2 ± 2.4 days for the MAb 1.2 group. At this dose, the groupsreceiving both MAbs lived significantly longer than the IgM anduntreated control groups (P $<=$ 0.0004, Kaplan-Meier log-rank survivaltest), and survival of the group receiving MAb 1.2 was greaterthan that of the group receiving MAb 1.10 (P = 0.016). For the1-µg dose, mean survival was 1.9 ± 0.1 days for the PBS group,2.2 ± 0.2 days for the control IgM group, 2.1 ± 0.1 days for theMAb 1.10 group, and 8.1 ± 1.9 days for the MAb 1.2 group. At thisdose, survival was significantly greater for the group receivingMAb 1.2 than the other groups (P $<=$ 0.017). All mice survivingto day 21 postinfection were alive 3 months postinfection. Protectionexperiments were performed two times with similar results.

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FIG. 3. Survival of CBA/N mice after infection with serotype 3 S. pneumoniae. (A) Survival of mice treated with MAb doses of 10 µg; (B) survival of mice treated with mAb doses of 1 µg. The y axes show percentages of mice surviving the number of days after infection depicted on the x axes. Mice were infected as described in the text after the administration of IgM (depicted by ×), PBS (#), MAb 1.2 (

), or mAb 1.10 ( $open circle$ ). The experiments were performed twice, and the results of one experiment are shown. In panel A, IgM (x) and PBS (#) had identical survival.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Our data show that XenoMouse animals vaccinated with a pneumococcal vaccine produced fully human antibodies to PPS antigensin the vaccine and that MAbs to PPS 3 generated from lymphocytesof PPS-vaccinated animals were protective in mice against serotype3 infection. XenoMouse mice are transgenic mice reconstitutedwith human immunoglobulin loci and inactivated endogenous heavyand kappa light-chain loci. The lambda loci of the animals areintact. Previous work with these mice has shown that the sizeof their immunoglobulin loci, which contain 66 V_H and 32 V $kappa$ genes,promotes both B-cell development (20) and human antigen-specificantibody responses (29). Whereas the latter had been shown onlyfor protein antigens, this report is the first to demonstratethat the XenoMouse repertoire is sufficient to generate an antipolysaccharideresponse. More work is needed to establish how closely the anti-PPSresponse of XenoMouse mice resembles that of humans, since therepertoire of XenoMouse mice does not contain a human $lambda$ locusand the $lambda$ light chain contributes to the human antibody responseto PPS (27, 32). However, our finding that like antibodiesto PPS from humans (3, 25, 27, 40), XenoMouse-derivedMAbs to PPS 3 use V_H3 genes suggests that the anti-PPS responsein these animals is restricted to V_H3 as it is inhumans.

Our data show that the antibody repertoire of XenoMouse animals is sufficient to generate fully human antibodies to PPS antigens.Similar to humans, the mice responded differently to differentserogroups, with the greatest response to PPS 3. This is interestingin light of data showing that PPS 3 was immunogenic in infants,whereas serogroups 6 and 19 were not (7). Although our findingssuggest a possible parallel with the responses of young childrento PPS serotypes (15), our studies were not designed to comparethe immunogenicities of different PPSs in the mice or to directlycompare the responses of the mice and humans. PPS is a weak immunogenwhich elicits a T-independent type 2 response (30), though ithas been noted that the adult response to some serotypes resemblesa recall response (27). Since environmental, cross-reactiveantigens and/or exposure to pneumococcal serotypes are proposedto play a role in establishing the antibody repertoire to PPS(27, 36), more work is necessary to determine whether andhow the preimmune repertoire influences the responses of XenoMousemice to certain PPSs, e.g., 6B and 19F. At present, the serotype-to-serotypeand mouse-to-mouse variability observed in the response to thePPS serotypes examined in this study is not understood. A factorwhich could contribute is that the sera were evaluated after multiplevaccinations. It has been reported that antibody levels to PPSantigens can be reduced in the presence of high concentrationsof polysaccharide (6) and the amount of vaccine administeredand its clearance may have varied for different PPSs among themice.

Reports from several groups show that V_H3 genes are used in the antibody responses to PPS (3, 27, 39, 40, 46).Our finding that the PPS 3-specific XenoMouse-derived MAbs expressedV_H3 genes lends further support to the concept of restrictionin the human anti-PPS response. A mechanism to explain this phenomenonhas not been described. V_H3 is the largest and most prevalenthuman V_H gene family subgroup, though its representation in theexpressed antibody repertoire has been attributed to antigen selectionin addition to the size of the subgroup (14). In this regard,it is noteworthy that common structural characteristics have beenfound among antibodies to defined types of antigens, e.g., polysaccharides(44), suggesting the possibility that only certain immunoglobulinreceptors can bind to polysaccharides. Consistent with the latter,V_H3 immunoglobulin receptors have unique structural characteristicswhich place them in a separate clan (clan III) and distinguishthem from the immunoglobulin receptors derived from other V_H subgroups(24). Interestingly, human antibodies to other capsular polysaccharides,namely, H. influenzae and Cryptococcus neoformans, also use V_H3genes (3, 4, 34).

V_H3 gene use alone appears to be insufficient to confer PPS specificity. DP 38/V3-15 was used in both the PPS3-specific MAb1.10 and human MAbs to PPS 8 and 6B (40, 46) as well as inthe nonspecific XenoMouse MAbs 1.1 and 2.1 and Fabs from a humancombinatorial library that cross-react with PVX, phosphorycholine,and DNA (25). The fact that the XenoMouse-derived MAbs weregerm line encoded indicates that the diversity generated by recombinationaland combinatorial mechanisms was sufficient to produce antibodiesspecific to PPS 3. A major influence on antibody specificity isthought to be the structure of antigen-antibody contact regions,particularly the CDR 3 which is created by a unique V-DJ joiningevent in each B cell (37). The PPS 3-specific MAbs 1.10, 1.2,and 1.4 had distinct CDR 3 regions and different avidity for PPS3. However, each MAb had a positively charged residue at V_H position94, as did the protective MAb described by Shaw et al. (39),whereas the nonspecific MAbs did not (Table 2). Such residueshave also been found in antibodies to DNA (25), suggesting thatcharge interactions may play a role in binding to negatively chargedmolecules. The frequency of CDR 3-encoded aromatic residues inthe PPS 3-specific XenoMouse-derived MAbs is consistent with theconcept that aromatic amino acids may enhance binding to capsularpolysaccharides (42, 45). However, a fuller understandingof the contribution of charge, polarity, and aromaticity to PPS3-antibody interactions must await formal structure-function analysisand/or crystallographicstudies.

Four of the XenoMouse-derived MAbs, including two that were specific for PPS 3 (MAbs 1.2 and 1.4), used V $kappa$ 1 genes. While ithas been suggested that certain cationic V $kappa$ 1 light chains mightpreferentially bind to negatively charged molecules, e.g., DNAand capsular polysaccharides (38, 41), this concept requiresfurther investigation. The use of proximal V $kappa$ genes is consistentwith previous studies of the antibody repertoires of XenoMousemice (29) and humans (13). The mice were reconstituted with32 J $kappa$ -proximal $kappa$ genes, which represent about 95% of the expressed $kappa$ genes in the human antibody repertoire (13). Thus, the PPS-elicitedlight-chain antibody repertoire in the mice resembled the naturallyoccurring human antibody repertoire. Consistent with other studies(25, 27) but in contrast to antibodies to H. influenzae (5,16), we did not find a predilection for expression of certainlight chains in the anti-PPS 3 response. Interestingly, a humanMAb to PPS 3 reported by the Shaw group (HU AB 14-3 [39]) alsoused a V $kappa$ CDR 3 motif QQ--S-P-T motif. Although the significanceof this motif for PPS 3 binding is uncertain, its existence inboth XenoMouse- and human-derived MAbs that were protective againstserotype 3 is intriguing. Lambda genes are used in antibodiesto PPS 6B (27, 40) and the polyreactive MAb to PPS 3 reportedby Shaw et al. (39). The significance of $lambda$ use by MAb 1.10 isuncertain since this MAb had an unexpressed V $kappa$ 2/A27 transcript,and the XenoMouse animals used in our studies lacked a human $lambda$ locus. Hence, the importance of the human $lambda$ repertoire in theanti-PPS response cannot be examined in thismodel.

The XenoMouse-derived MAbs 1.10 and 1.2 were protective in mice. This is a significant finding, since some human antibodiesenhanced pneumococcal infection in mice (2, 35). MAb 1.2was more effective than MAb 1.10 in that it mediated survivalof a greater proportion of animals at a 10-fold-lower dose. Sincecomplement opsonins enhance antibody-mediated opsonization ofS. pneumoniae (11) and are required for IgM-mediated protectionagainst the pneumococcus (46), the greater complement depositionon PPS 3 mediated by MAb 1.2 may be a correlate of its superiorprotective efficacy. However, other mechanisms such as phagocytosisof antigen-antibody aggregates may also play a role in IgM-mediatedprotection (31). The use of different genetic elements and theunique CDR 3 sequences of MAbs 1.10 and 1.2 raise the possibilitythat they had differences in fine specificity which translatedinto differences in biological activity. Alternatively, MAb 1.10may have had a reduced ability to activate complement and/or differentpharmacokinetics because it expressed a mouse $lambda$ . Thus, furtherstudies are needed to fully understand the observed differencesin the protective efficacy of MAb 1.10 as compared to MAb 1.2.

In summary, our data demonstrate that XenoMouse mice produced protective antibodies to PPS 3 that use V_H3 genes. The germline configuration of the MAbs indicates that the antibody repertoireof these animals is sufficient to generate an anti-PPS 3 responsewhich reflects the V_H usage of the native human repertoire. Thestudy of human antibodies to PPS in the XenoMouse model has thepotential enlarge the basic science knowledge base regarding themolecular characteristics of protective antibodies to S. pneumoniae.Such information is likely to provide insight into possible mechanismsof vaccine failure and facilitate the development of new approachesto treating and preventing pneumococcalinfections.

	ACKNOWLEDGMENTS

This work was supported by NIH grant AI 35370 to L.P. and NIH Microbial Pathogenesis Training Grant 1 P32 AI 07506 to N.D.R.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Infectious Diseases, Albert Einstein College of Medicine, 1300 Morris ParkAve., Room 402 Forchheimer Building, Bronx, NY 10461. Phone: (718)430-2372. Fax: (718) 430-8968. E-mail: pirofski{at}aecom.yu.edu.

Editor: T. R. Kozel

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