Pneumococcal Type 22F Polysaccharide Absorption Improves the Specificity of a Pneumococcal-Polysaccharide Enzyme-Linked Immunosorbent Assay

doi:10.1128/CDLI.8.2.266-272.2001

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Clinical and Diagnostic Laboratory Immunology, March 2001, p. 266-272, Vol. 8, No. 2
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.2.266-272.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Pneumococcal Type 22F Polysaccharide Absorption Improves the Specificity of a Pneumococcal-Polysaccharide Enzyme-Linked Immunosorbent Assay

Nelydia F. Concepcion and Carl E. Frasch^*

Laboratory of Bacterial Polysaccharides, Center for Biologics Evaluation and Research, Bethesda, Maryland

Received 24 July 2000/Returned for modification 9 October 2000/Accepted 21 November 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The specificity of the immune response to the 23-valent pneumococcal-polysaccharide (PS) vaccine in healthy adults and toa pneumococcal conjugate vaccine in infants was examined by measuringimmunoglobulin G (IgG) antibody titers by enzyme-linked immunosorbentassay (ELISA) and the opsonophagocytosis assay. ELISA measurestotal antipneumococcal IgG titers including the titers of functionaland nonfunctional antibodies, while the opsonophagocytosis assaymeasures only functional-antibody titers. Twenty-four pairs ofpre- and post-pneumococcal vaccination sera from adults were evaluated(ELISA) for levels of IgG antibodies against serotypes 4, 6B,9V, 14, 18C, 19F, and 23F. Twelve of the pairs were also examined(opsonophagocytosis assay) for their functional activities. Thecorrelation coefficients between assay results for most typesranged from 0.75 to 0.90, but the correlation coefficient wasonly about 0.6 for serotypes 4 and 19F. The specificities of theseantibodies were further examined by the use of competitive ELISAinhibition. A number of heterologous polysaccharides (types 11A,12F, 15B, 22F, and 33A) were used as inhibitors. Most of the seratested showed cross-reacting antibodies, in addition to thoseremoved by pneumococcal C PS absorption. Our data suggest thepresence of a common epitope that is found on most pneumococcalPS but that is not absorbed by purified C PS. Use of a heterologouspneumococcal PS (22F) to adsorb the antibodies to the common epitopeincreased the correlation between the IgG ELISA results and theopsonophagocytosis assay results. The correlation coefficientimprove from 0.66 to 0.92 for type 4 and from 0.63 to 0.80 fortype 19F. These common-epitope antibodies were largely absentin infants at 7 months of age, suggesting the carbohydrate natureof theepitope.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Streptococcus pneumoniae (pneumococcus) is now the leading cause of invasive bacterial disease in children under the age of5 years. Although there are 90 different pneumococcal serotypesbased upon the presence of chemically and immunologically differentcapsular polysaccharides (PSs), most pneumococcal disease in youngchildren in many countries is caused by less than 12 of thesetypes (7, 8).

The newly U.S. licensed Wyeth Lederle Vaccines seven-valent pneumococcal conjugate vaccine, called Prevnar, containing PStypes 4, 6B, 9V, 14, 18C, 19F, and 23F, was shown to be highlyeffective in reducing the incidence of invasive pneumococcal diseasein infants and children under 2 years of age (2, 16). Otherpneumococcal conjugate vaccines are in clinical trials (7).These include the 9- and 11-valent formulations, which add types1 and 5 and types 1, 3, 5, and 7F, respectively. These vaccineswill need to be evaluated for safety and efficacy. The ideal studydesign for evaluation of the efficacies of these vaccines is determinationof the incidence of pneumococcal disease in a vaccinated groupagainst the incidence in a nonvaccinated control group, but suchtrials may be very difficult. Thus, there is a need for in vitroantibody assays that can strongly predict protectiveefficacy.

Protection against invasive pneumococcal disease is mediated by the presence of opsonic antibodies (12, 22). Both thepneumococcal PS and conjugate vaccines induce type-specific opsonicantibodies (12, 20). Thus, in vitro measurements of opsonophagocytosismay serve as a surrogate for protection. However, opsonophagocytosisassays are labor-intensive and difficult to perform with largenumbers of samples. Thus, many laboratories measure antibody bindingonly by enzyme-linked immunosorbent assay (ELISA). Since clinicalprotection against pneumococcal infection is mediated by antibodiesto the capsular PS, an ELISA that measures immunoglobulin G (IgG)antibody levels may be used in place of opsonophagocytosis assays,provided that a sufficient correlation between the two assayscan beshown.

Antibody concentrations and the role of antibody avidity in protection from pneumococcal infections are unclear, but previousstudies with Haemophilus influenzae type b conjugate vaccineshave shown that high-avidity antibodies perform better on a weightbasis in bactericidal assays and are more protective against experimentalinfection (11).

The present study focused on two important aspects of an immunological assay: specificity and correlation of binding antibodiesto functional activity. Purified capsular PSs contain approximately5% (by weight) contaminating C PS, some of which is covalentlybound to the type-specific PS through a peptidoglycan fragment(19). While children and adults have naturally acquired antibodiesto the C PS (10), these antibodies are not opsonic and do notprotect against pneumococcal infection (14, 21). Therefore,such antibodies should be blocked so that only the levels of antibodiesspecific to the C PS are measured (13, 20). Other investigatorshave shown that pneumococcal C PS preparations may also containnon-C PS contaminants that are immunogenic (18, 23). The studiesreported here will show the presence of a common epitope in additionto the C PS shared among several pneumococcal PS types and thatantibodies to this common epitope are not absorbed by solubleC PS but are removed by using pneumococcal type 22F PS as a secondabsorbant. Following removal of these additional antibodies, theresulting IgG concentrations correlate more highly with the titersdetermined by opsonophagocytosisassays.

	MATERIALS AND METHODS

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Sera and reagents. Sera obtained before and after immunization of 12 adults with a 23-valent pneumococcal PS vaccine were provided by David Goldblatt,Institute of Child Health, London, United Kingdom. Sera from healthyadults were from our laboratory's serum bank. Postvaccinationsera from infants who had received three doses of a tetravalent(types 6B, 14, 19F, and 23F) pneumococcal conjugate vaccine werekindly provided by Merck & Company, West Point,Pa.

The pneumococcal PSs and HL-60 cells were obtained from the American Type Culture Collection (ATCC), Manassas, Va. C PS wasobtained from the State Serum Institute, Copenhagen, Denmark.The alkaline phosphatase-labeled anti-IgG antibodies and substratetablets were obtained from Sigma Chemical Company, St. Louis,Mo. The complement source for the opsonophagocytosis assays wasserum from 3- to 4-week-old rabbits (Pel-Freeze, Brown Deer, Wis.).The Centers for Disease Control and Prevention (Atlanta, Ga.)provided the bacterial strains used in the phagocytosis assays.RPMI 1640, penicillin-streptomycin solution, and Hank's balancedsalt solution with and without Ca²⁺ and Mg²⁺ were obtained from Life Technologies, Grand Island, N.Y. Fetalcalf serum was bought from Hyclone Laboratories, Logan, Utah.Todd-Hewitt broth, yeast extract, Bacto Agar, and gelatin werepurchased from Difco, Detroit,Mich.

ELISA. Optimal concentrations of pneumococcal PS and methylated human serum albumin were determined to obtain the highest specificbinding to Immulon no. 1 ELISA plates and ranged from 1.0 to 5.0µg/ml for the PS and 0.5 to 5.0 µg/ml for methylated human serumalbumin (4). Coated plates were then left at room temperaturefor 6 to 16 h. The ELISA was performed as described previously(4).

Inhibition ELISA. Competitive inhibition ELISA (6) was performed by diluting serum samples in serum conjugate buffer containing 1 µg of CPS per ml plus various concentrations (0.04 to 2.0 µg/ml) of oneof five other pneumococcal PS types, type 11A, 12A, 15B, 22F,and 33F PSs. These PSs are present in the 23-valent vaccine butnot in the 7-, 9-, or 11-valent conjugate vaccines currently underinvestigation (7). These PSs have no known cross-reactivitywith other pneumococcal PS serogroups (8). PS type 22F wasselected because it gave somewhat better absorption compared tothe absorptions for the other pneumococcal PS types tested. Theoptimal concentration was found to be 1.0 µg/ml for C PS absorptionand 2.0 µg/ml for PS type 22F absorption. All the serum samplestested were diluted in serum-conjugate buffer containing C PSand PS type 22F. The remainder of the ELISA procedure was as describedpreviously (4).

Opsonophagocytosis assay. Cells of the HL-60 cell line, a human continuous lymphoblastic cell line were rather than traditional polymorphonuclear leukocytesused as the effector cells. HL-60 cells undergo granulocytic differentiationupon chemical induction for 7 to 10 days with dimethyl formamide.The procedure followed was that previously described by Romero-Steineret al. (17). Opsonophagocytosis assay titers were expressedas the reciprocal of the highest serum dilution that killed $>=$ 50%of the organisms compared to the number of organisms in the complementcontrol wells. Serum samples were tested beginning at a dilutionof 1:8. Samples with a titer lower than 1:8 were considered negative,and the results are reported as a titer of 1:4 for purposes ofdataanalysis.

Statistical analysis. Correlation coefficients between the ELISA titers (in micrograms per milliliter) and the log₂ of the opsonophagocytosis assaytiters were calculated with the Instat computer program. A quadrantmethod of analysis, as described in the Results section, was alsoused to compare theassays.

	RESULTS

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Twelve pairs of serum samples from adults who were vaccinated with the 23-valent pneumococcal PS vaccine were analyzed byELISA for titers of IgG antibodies against the seven types containedin the seven-valent conjugate vaccine: types 4, 6B, 9V, 14, 18C,19F, and 23F. These same serum samples were then examined by theopsonophagocytosis assay with HL-60 cells. Correlation coefficientswere calculated between the two assays and gave a range from 0.63to 0.90, as shown in Table 1.

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TABLE 1. Correlation of ELISA and opsonophagocytosis assay for 12 pairs of pre- and postvaccination serum samples from adults^a

Sera from immunized or nonimmunized adults may have high antibody levels that are not PS specific and that are not absorbedwith soluble C PS (18, 23). Sera from four nonimmunized adultswere adsorbed with C PS plus the homologous PS type or one offive heterologous PS types and were examined on ELISA plates coatedwith type 9V PS (Fig. 1). The heterologous PSs were chosen becausethey are available from ATCC, are not presently included in anypneumococcal conjugate vaccine, and have no shared antigenic cross-reactivity(see Table 6 in reference 7). Adsorption with heterologouspneumococcal PSs reduced antibody binding to the homologous 9VPS. Of the four serum samples, serum sample 746 showed the desiredtype specificity, being strongly inhibited only by the homologousPS. The other three serum samples were strongly inhibited by allsix PSs and thus contained essentially no type 9V-specific antibodies.

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FIG. 1. Competitive ELISA inhibition of pneumococcal PS type 9V antibody with homologous (type 9V) and heterologous (type 11A, 12F, 15B, 22F, and 33F) pneumococcal PSs. The inhibitors were used at 10 µg/ml.

Sera without evident type-specific antibodies are not opsonic. We selected two serum samples with antibody concentrationssimilar to those for type 19F following C PS absorption; one wasstrongly opsonic for type 19F and the other was nonopsonic. Thesetwo serum samples were then absorbed by the homologous type 19FPS or one of three heterologous pneumococcal PSs and were thenexamined by ELISA (Fig. 2). Only the type 19F PS removed antibodiesto type 19F in the opsonic serum sample, while all four PSs equallyabsorbed the binding antibody in the nonopsonic serum sample.Thus, antibodies are present to an antigen that is common to thesepneumococcal types that are not PS type specific and not opsonic.

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FIG. 2. Specificities of antibodies reactive with pneumococcal type 19F PS following C PS absorption. (A) Results for a serum sample from an adult that had 6.6 µg of type 19F IgG per ml and that was functional by opsonophagocytosis assay. Heterologous pneumococcal PSs of types 1, 4, and 6B were used as inhibitors. The results for the homologous pneumococcal PS, the type 19F PS, is indicated by the broken line. (B) Results for a serum sample from an adult that had 7.7 µg of IgG to type 19F per ml but that was not opsonic for type 19F. OD, optical density; Pn, pneumococcal PS type.

From the data presented in Fig. 1 the pneumococcal type 22F PS was selected for further evaluation as a second absorbent.Assays were performed to determine the appropriate concentrationof type 22F PS to be included in the serum dilution buffer. Aserum sample with a large proportion of antibodies to the commonantigen was used, and the amount of type 22F PS needed to achievemaximal inhibition of antibodies to the common antigen was determinedfor seven pneumococcal PS types (Fig. 3). Near-optimal inhibitionwas achieved with about 1 µg of the type 22F PS per ml for sixof the types. In contrast, type 22F absorption had no effect onbinding of antibody to the type 14 PS. We chose to use 2 µg ofthe type 22F PS per ml to account for possible lot-to-lot differencesin the common cross-reactive component.

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FIG. 3. Determination of optimal type 22F PS concentration for use as an inhibitor. Competitive inhibition with type 22F PS on antibody binding in a serum sample from a healthy adult was done for the seven pneumococcal PS types present in the seven-valent conjugate vaccine. Pn, pneumococcal PS type.

Figure 4 shows the relative effect of C PS absorption compared to that of C PS plus type 22F PS absorption on antibodies measuredin a serum sample from a healthy adult against 11 pneumococcaltypes considered for inclusion in conjugate vaccines. Most ofthe cross-reactive antibodies were removed by the C PS, with furthersmaller reductions obtained by the double absorption. The notableexceptions were types 3 and 14, in which type 22F absorption hada minimal effect on the estimated antibody concentrations.

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FIG. 4. Comparative effects of C PS absorption and combined C PS and type 22F PS absorption on a serum sample from an unimmunized adult for 11 pneumococcal types. The C PS and type 22F PS were used at 1 and 2 µg/ml, respectively.

A batch of serotype 22F PS obtained from Merck & Company (Merck & Company supplies the pneumococcal PSs distributed by ATCC)was compared to two other batches of type 22F PS; one was fromATCC and another one was from Wyeth Lederle Vaccines. When presentat 2 µg/ml in the serum dilution buffer, all were equally effectiveat removing the additional antibodies (data notshown).

The overall effect of the added type 22F PS absorption on sera from adults pre- and postimmunization with the 23-valent PSvaccine is shown in Fig. 5. The mean percent reduction in antibodybinding by type 22F PS for 10 preimmunization serum samples and18 postimmunization serum samples is shown for 11 pneumococcaltypes. As expected, the proportion of type-specific antibodieswas greater postimmunization. Again, there was no effect of type22F absorption on antibody binding to type 14 and relatively littleeffect on antibody binding to type 3. In contrast to adults, infantsat 7 months of age have little or no common antigen-reactive antibodiesfollowing immunization with a pneumococcal conjugate vaccine (Fig.6). Data for type 6B are shown, and similar data were obtainedfor type 23F.

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FIG. 5. Percent reduction of IgG antibody binding in pre- and postvaccination sera following type 22F PS absorption. The mean percent reduction for 10 preimmunization serum samples and 18 postimmunization serum samples are given for 11 pneumococcal types. Percent reduction was calculated as ([IgG] with C PS absorption only $-$ [IgG] with C PS and 22F absorption)/ [IgG] with C PS absorption only × 100.

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FIG. 6. Percent reduction in antibody binding to the type 6B PS by using type 22F PS absorption in postimmunization sera from seven 7-month-old infants. Percent reduction was calculated as described in the legend to Fig. 5.

Absorption with C PS plus the type 22F PS removes nonserotype-specific and nonopsonic antibodies, improving the correlationbetween the IgG antibody concentrations measured by ELISA andthe opsonophagocytosis assay titers. This effect is illustratedfor types 4 and 19F (Fig. 7 and 8, respectively). Antibody concentrationsversus opsonophagocytosis assay titers were examined by a quadrantanalysis. For this analysis, the upper left-hand quadrant representsthe number of serum samples which are opsonic and which have $<=$ 1.0µg of IgG per ml as determined by ELISA. The upper right quadrantrepresents those sera samples that are both opsonic and have IgGconcentrations >1.0 µg/ml. The lower left quadrant contains thenonopsonic serum samples with $<=$ 1.0 µg of IgG per ml, and the lowerright quadrant contains the number of serum samples that are nonopsonicbut that have IgG concentrations of >1.0 µg/ml. Ideally, thereshould be no datum points in the upper left and lower right quadrants.For type 4, absorption with type 22F reduced the number of nonopsonicserum samples with IgG levels >1 µg/ml from 10 to 1 (Fig. 7).The correlation coefficient increased from 0.66 to 0.92. Similarlyfor type 19F, after type 22F absorption, the number of nonopsonicserum samples with IgG concentrations >1 µg/ml was reduced from12 to 5 and the correlation coefficient improved from 0.63 to0.80 (Fig. 8).

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FIG. 7. Correlation of pneumococcal type 4 ELISA and opsonophagocytosis assay titers. (A) After C PS absorption only. (B) After C PS plus type 22F PS absorption. The quadrant lines were drawn at the 1.0-µg/ml cutoff for ELISA and the log₂ (1:4) cutoff for the opsonophagocytosis assay titer. The numbers shown are the number of serum samples in each quadrant. The r values were 0.66 before type 22F PS absorption and 0.92 after type 22F PS absorption.

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FIG. 8. Correlation of pneumococcal type 19F ELISA and opsonophagocytosis assay titers. (A) After C PS absorption. (B) After C PS plus type 22F PS absorption. The quadrant lines were drawn at the 1.0 µg/ml cutoff for the ELISA titer and the log₂ (1:4) cutoff for the opsonophagocytosis assay titer. The r value was 0.63 before type 22F PS absorption and 0.80 after type 22F PS absorption.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Protection against pneumococcal bacteremia, pneumonia, or otitis media is mediated by antibodies that are opsonic (12).Pneumococcal PSs are immunogenic and induce type-specific protectiveimmunity. Thus, in vitro measurement of opsonophagocytosis byanti-PS antibodies is a surrogate measure of clinical protection.However, due to the difficulties of measuring opsonic antibodytiters in large numbers of vaccinees, many laboratories use antibodybinding assays, usually ELISA (4, 9).

The pneumococcal cell wall contains a number of carbohydrate structures. All pneumococci express C PS. The C PS is covalentlylinked to the peptidoglycan and is composed of a tetrasaccharidesubunit linked through a phophodiester linkage. It is closelyrelated to the lipoteichoic acid F antigen (19). In encapsulatedpneumococci the C PS is covalently linked to the type-specificPS. The nature of the attachment is not known, but it may be analogousto the reported association of the group B carbohydrate and type-specificcapsular PS of Streptococcus agalactiae (5). Here, both thegroup-specific and the type-specific antigens are covalently linkedto the peptidoglycan, but to differentsugars.

The pneumococcal PS antigens used in the ELISA contain about 5% (by weight) of C PS as a contaminant. All individuals includinginfants have antibodies to the C PS as a result of early exposureto pneumococci and Streptococcus mitis (U. B. S. Sorensen, N.Bergstrom, C. Karlsson, M. Killian, and P. E. Jansson, SecondInt. Symp. Pneumococci Pneumococcal Dis. abstr., 2000). The concentrationsof antibody to the C PS in unimmunized individuals often exceedthose of antibody to the type-specific PSs (Fig. 4). Thus, thecurrent pneumococcal ELISA protocols have an absorption step toremove C PS antibodies (4, 9, 10).

For an ELISA to be used in place of an opsonophagocytosis assay, there should be a strong correlation between the measuredantibody concentration and opsonic antibody titers. Thus, theELISA method should be PS type specific (see below) and correlatewell with functional activity (we suggest an r value of $>=$ 0.8 combinedwith a quadrant analysis). Human antibodies to the pneumococcalC PS are not opsonic (20), and the antibody concentrations measuredwithout removal of these antibodies showed no correlation betweenthe amount of IgG bound and the opsonophagocytosis assaytiter.

The specificity of the PS ELISA for a given serotype after removal of C PS antibodies was assessed by inhibition with homologousand heterologous pneumococcal PSs. We consider that there shouldbe <20% inhibition by heterologous PS types, but some sera fromhealthy nonimmunized adults were found for some types to be nearlyequally inhibited by homologous and heterologous pneumococcalPSs. Such sera were often found to be devoid of opsonic antibodiesto that type. Yu et al. (23) found that some postvaccinationsera positive for pneumococcal PS were much less opsonic for type6B than would have been predicted from the type 6B antibody concentrationsmeasured by ELISA and that a heterologous PS, type 9V PS, removedmost of the nonopsonic antibodies. These observations indicatethat absorption with the highly purified soluble C PS alone isnot sufficient to remove all common cross-reactive antibodies.Yu et al. (23) stated that the novel epitope was distinct fromthe C PS, but as outlined below, our working hypothesis is somewhatdifferent.

Another conclusion from the cross-absorption experiments was that the purified pneumococcal type PSs contained another commonantigen in addition to the C PS. Our working hypothesis is thatthis additional common epitope is actually the linkage regionbetween the C PS and the type-specific PS, and this region cannotbe present in the highly purified soluble C PS, which is isolatedfrom a rough pneumococcal strain with a C PS capsule (3, 15).In support of this hypothesis was the observation by Yu et al.(23) that a lysate from a nonencapsulated pneumococcal strainwas less able to inhibit the cross-reactive antibody than a lysatefrom an encapsulated strain. It is further supported by the observationby Soininen et al. (18) that the cross-reactive antibodies thatremain after C PS absorption were predominantly of the IgG2 subclass,implying that these cross-reactive antibodies were directed againsta PS determinant. Furthermore, Bornstein et al. 3 demonstratedantigenic heterogeneity among C PSpreparations.

The pneumococcal 11-valent conjugate vaccines under clinical investigation contain types 1, 3, 4, 5, 6B, 7F, 9V, 14, 18C,19F, and 23F (7). The licensed 23-valent PS vaccine contains12 additional types, and from these additional types we selectedfor evaluation as a possible second absorbent types 11A, 12F,15B, 22F, and 33F, as these types are not included in any presentconjugate vaccine, they lack shared type-specific epitopes withother pneumococcal serogroups (8), and they are available fromATCC. Although we chose type 22F, type 22F was not materiallydifferent from the other four types tested. Yu et al. (23) havereported that type 9V also contains substantial amounts of a commonantigen. However, absorption with the heterologous PS alone couldnot replace absorption with soluble C PS (C. E. Frasch, unpublishedobservations).

An important observation was that the antibodies against common epitopes were present in sera from all adults tested but wererarely observed in sera from 7-month-old infants, either thosewho were vaccinated with the pneumococcal conjugate or those whowere nonvaccinated. This suggests that the common antigen is carbohydratein nature. By contrast, by 7 months of age most all infants hadmeasurable antibodies to the soluble C PS, as C PS absorptionreduced antibody binding to the type-specific PS-coated ELISAplates. The ubiquitous presence of C PS on such commensals asStreptococcus mitis may explain the presence of C PS antibodiesin theinfants.

In order to be used in place of functional assays, the results of an ELISA method should, at a minimum, correlate well (r $>=$ 0.8) with those of the opsonophagocytosis assay. We also recommendthat the data be examined visually (for example, by quadrant analysis)to evaluate the number of individual serum samples with discordantresults. The correlation between antibody binding by ELISA andopsonphagocytosis assay for 24 serum samples from adults is shownin Table 1. Serotypes 4 and 19F showed the weakest correlationwhen the sera were absorbed only with C PS. Removal of additionalnonopsonic antibodies by type 22F absorption increased the correlationcoefficients between antibody binding and opsonophagocytic assaytiters for types 4 and 19F from 0.66 and 0.63 before type 22Fabsorption to 0.92 and 0.80 after type 22F absorption. Thus, combinedC PS and type 22F PS absorption increases the type specificityand improves the correlation with functionalactivity.

Although the thrust of our work has been to improve the specificity in measurement of pneumococcal vaccine-induced antibodytiters in healthy individuals, retrieval of optimal pneumococcalantibody specificity in sera from patients, including immunocompromisedindividuals, is also important, because these individuals mayhave high levels of common antigen-reactive antibodies, whichdo not appear to contribute toprotection.

In conclusion, we have found that absorption with a heterologous pneumococcal PS blocks binding of nonopsonic antibodies andby so doing have made the PS ELISA more predictive of functionalactivity. On the basis of the results presented in this report,we recommend that sera be absorbed with both C PS and type 22FPS, recognizing that the type 22F PS was not materially superiorto other heterologous PS types evaluated. Additional studies areneeded to examine the age-related acquisition of the common antigenantibodies. We are investigating whether the linkage region ofthe C PS to the type-specific PS carries the commonepitope.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Bacterial Products, CBER, 1401 Rockville Pike, HFM-428, Rockville, MD 20852.Phone: (301) 496-1920. Fax: (301) 402-2776. E-mail: frasch{at}cber.fda.gov.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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18. Soininen, A., G. Dobbelstein, L. Oomen, and H. Kayhty. 2000. Are the enzyme immunoassays for antibodies to pneumococcal capsular polysaccharides type specific? Clin. Diagn. Lab. Immunol. 7:468-476[Abstract/Free Full Text].

19. Sorensen, U. B. S., J. Henrichsen, H.-C. Chen, and S. C. Szu. 1990. Covalent linkage between the capsular polysaccharide of Streptococcus pneumoniae revealed by immunochemical methods. Microb. Pathog. 8:325-334[CrossRef][Medline].

20. Vioarsson, G., I. Jónsdóttir, S. Jónsson, and H. Valdimarsson. 1994. Opsonization and antibodies to capsular and cell wall polysaccharides of Streptococcus pneumoniae. J. Infect. Dis. 170:592-599[Medline].

21. Watson, D. A., and D. M. Musher. 1993. Assessment of responses to pneumococcal infection and vaccination using enzyme-linked immunoassay. Serodiagn. Immunother. Dis. 5:131-133.

22. Winkelstein, J. A. 1981. The role of complement in the host's defense against Streptococcus pneumoniae. Rev. Infect. Dis. 3:289-298[Medline].

23. Yu, X. H., Y. Sun, C. Frasch, N. Concepcion, and M. H. Nahm. 1999. Pneumococcal capsular polysaccharide preparations may contain non-C-polysaccharide contaminants that are immunogenic. Clin. Diagn. Lab. Immunol. 6:519-524[Abstract/Free Full Text].

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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.	Infect. Immun.
J. Clin. Microbiol.	J. Virol.	ALL ASM JOURNALS

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19.	Sorensen, U. B. S., J. Henrichsen, H.-C. Chen, and S. C. Szu. 1990. Covalent linkage between the capsular polysaccharide of Streptococcus pneumoniae revealed by immunochemical methods. Microb. Pathog. 8:325-334[CrossRef][Medline].
20.	Vioarsson, G., I. Jónsdóttir, S. Jónsson, and H. Valdimarsson. 1994. Opsonization and antibodies to capsular and cell wall polysaccharides of Streptococcus pneumoniae. J. Infect. Dis. 170:592-599[Medline].
21.	Watson, D. A., and D. M. Musher. 1993. Assessment of responses to pneumococcal infection and vaccination using enzyme-linked immunoassay. Serodiagn. Immunother. Dis. 5:131-133.
22.	Winkelstein, J. A. 1981. The role of complement in the host's defense against Streptococcus pneumoniae. Rev. Infect. Dis. 3:289-298[Medline].
23.	Yu, X. H., Y. Sun, C. Frasch, N. Concepcion, and M. H. Nahm. 1999. Pneumococcal capsular polysaccharide preparations may contain non-C-polysaccharide contaminants that are immunogenic. Clin. Diagn. Lab. Immunol. 6:519-524[Abstract/Free Full Text].