Up-Regulation of CD40 Ligand and Induction of a Th2 Response in Children Immunized with Pneumococcal Polysaccharide Vaccines

doi:10.1128/CDLI.8.2.233-240.2001

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Clinical and Diagnostic Laboratory Immunology, March 2001, p. 233-240, Vol. 8, No. 2
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.2.233-240.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Up-Regulation of CD40 Ligand and Induction of a Th2 Response in Children Immunized with Pneumococcal Polysaccharide Vaccines

Lily E. Leiva,^* Boyd Butler, James Hempe, Alejandro P. Ortigas, and Ricardo U. Sorensen

Department of Pediatrics, Louisiana State University Health Sciences Center and Children's Hospital, New Orleans, Louisiana

Received 19 July 2000/Returned for modification 28 August 2000/Accepted 15 November 2000

	ABSTRACT

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We wished to determine whether pneumococcal polysaccharide antigens induce mRNA expression of CD40 ligand (CD40L) and Th1or Th2 cytokines in unimmunized individuals in vitro and whetherimmunization with the 23-valent pneumococcal polysaccharide vaccineinduces changes in CD40L and cytokine mRNA expression. Childrenwith recurrent respiratory infections were studied before and4 to 6 weeks after receiving the pneumococcal vaccine. One patientwho failed to respond to the polysacharide vaccine subsequentlyreceived a single dose of the experimental 7-valent pneumococcalconjugate vaccine. Unimmunized healthy adults were included ascontrols. Quantification of mRNA expression of CD40L, interleukin-4(IL-4), IL-12p40, and gamma interferon (IFN- $gamma$ ) was performed byreverse transcription-PCR and enzyme-linked immunosorbent assay(ELISA)-PCR with resting and stimulated peripheral blood mononuclearcells. Serum immunoglobulin G (IgG) anti pneumococcal antibodylevels were measured by ELISA. The results showed a significantincrease in the expression of mRNAs for CD40L and IL-4, but notIL-12p40 or IFN- $gamma$ , in stimulated cultures from unimmunized individuals.CD40L and IL-4 mRNA expression was significantly higher in postimmunizationthan in preimmunization samples stimulated with the individualpneumococcal serotypes. These results suggest that pneumococcalpolysaccharide antigens specifically up-regulate CD40L expressionand induce a Th2 response in vitro which parallels the increasein IgG antipneumococcal antibody levels inserum.

	INTRODUCTION

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The immune response to vaccines, including polysaccharide vaccines, is evaluated by measuring the production of antibodiesagainst specific vaccine antigens in vivo. Polysaccharides arethymus-independent (TI) antigens, which, like thymus-dependent(TD) antigens, induce immunoglobulin secretion and immunoglobulinclass switching. However, the induction and mechanisms regulatingthe response to the polysaccharides appear to be different. Antibodyresponses to TD antigens require antigen-specific T-cell help,while TI antigens are known for their ability to stimulate antibodyproduction in T-cell-depleted mice in vivo and in T-cell-depletedcultures in vitro (3). TI antigens have been subdivided intotype 1 (TI-1) antigens, which have no T-cell interaction, andtype 2 (TI-2) antigens, which have some interaction with T cells.Recent studies have shown that pneumococcal polysaccharides areTI-2 antigens, which stimulate T-cell help in regulating antibodyproduction (11, 14, 20, 21, 31). However, neither theway in which such stimulation occurs nor the regulatory mechanismof antibody production is well understood. Regulatory molecules,such as CD40 ligand (CD40L) and cytokines, may play an importantrole in the antibody response to pneumococcalpolysaccharides.

CD40L is essential for the antibody response to TD antigens by inducing B-cell proliferation and isotype switching throughthe interaction with CD40 expressed on B cells (6, 7, 18,19). The role of CD40L in the immune response to TI-2 antigensis less clearly understood despite the observation that TI-2 antigensinduce CD40L expression in vivo (32).

Cytokines secreted by T helper (Th) cells play a critical role in antibody-mediated immune responses. The Th1 subset producesinterleukin-2 (IL-2) and gamma interferon (IFN $gamma$ ), which promotedelayed-type hypersensitivity, whereas the Th2 subset producesIL-4, IL-5, IL-10, and IL-13, which shift the immune responseto immunoglobulin G (IgG) and IgE antibody production (16, 17,22). The differentiation of naive T cells to either the Th1or Th2 subset is regulated by cytokines present at the time ofantigenic stimulation (12, 25). IL-12, a p70 heterodimer composedof 35- and 40-kDa subunits, is a regulatory cytokine producedby macrophages and B cells which stimulate Th1 differentiationin vitro and in vivo (4, 12).

Recent evidence indicates that TI-2 antigens are capable of inducing regulatory cytokines in the spleens of mice immunizedwith trinitrophenyl-Ficoll (5, 32). The role of CD40L andcytokines in the induction of an antibody response to pneumococcalvaccines has not been extensively studied inhumans.

Polysaccharide antigens are known to be poor immunogens in humans under 2 years of age. Furthermore, some patients with recurrentrespiratory infections fail to respond to polysaccharide antigensat any age (8, 23, 30, 35). This lack of response canbe overcome by conjugating the polysaccharide to a protein carrier.Several experimental pneumococcal conjugate vaccines have recentlybeen developed (1, 2, 9, 27). We have previously shownthat the CRM197-heptavalent pneumococcal conjugate vaccine inducedan IgG antibody response in patients with recurrent infectionswho had failed to mount an adequate response to the polysaccharidevaccine (28).

In the present study, we wished to determine whether pneumococcal polysaccharide antigens are able to induce mRNA expressionof CD40L and Th1 or Th2 cytokines in unimmunized individuals invitro and whether immunization with the 23-valent polysaccharidevaccine (23-PV) or the conjugate vaccine induces changes in CD40Land cytokine mRNA expression 4 weeks afterimmunization.

	MATERIALS AND METHODS

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Study population. We evaluated 15 patients (2 to 13 years of age) referred to our pediatric allergy-immunology clinic for evaluation of recurrentrespiratory infections. None of these patients had immunoglobulin,IgG subclass, or other known primary or secondary immunodeficiencies.They had all received routine immunizations, including DPT, requiredfor their ages (by history). As part of their evaluation, patientsreceived one does of a 23-valent pneumococcal polysaccharide vaccine(Pnu-Immune; Wyeth-Lederle, Pearl River, N.Y.). One patient whofailed to respond to 23-PV received a single dose of an experimental7-valent pneumococcal conjugate vaccine within 6 months of immunizationwith 23-PV after parental consent (28). Four unimmunized healthyadults were also included as controls. Serum concentrations ofantipneumococcal polysaccharide antibodies and mRNAs for CD40L,IL-4, IL-12p40, and IFN- $gamma$ extracted from in vitro-stimulated peripheralblood mononuclear cells (PBMC) were measured before and 4 to 6weeks after pneumococcal vaccination for patients and 4 weeksapart for the unimmunizedcontrols.

Experimental heptavalent pneumococcal conjugate vaccine. The experimental pneumococcal conjugate vaccine (supplied by Wyeth-Lederle) contains polysaccharide conjugates of serotypes4, 6B, 9V, 14, 19F, and 23F and an oligosaccharide conjugate ofserotype 18C produced by reactive amination. The carrier proteinfor all conjugates is CRM197, a nontoxic variant of diphtheriatoxin. This vaccine has recently been approved for use by theFood and Drug Administration(FDA).

Cell preparations and cultures. PBMC from 2 ml of blood were isolated by Ficoll-Hypaque (density, 1.077g/cm³; Sigma, St. Louis, Mo.) gradient centrifugation. After an overnightincubation in RPMI 1640 at 37°C in humidified air containing 5%CO₂, PBMC (5 × 10⁵) were cultured for 5 h in the absence or presence of concanavalinA (ConA) (20 mg/ml; Miles Scientific, Naperville Ill.), tetanustoxoid (TT) adsorbed USP (1:500; Connaught Laboratories Inc.,Swiftwater, Pa.), 23-PV (1:500; Pnu-Immune, Lederle-Praxis Biologicals),and pneumococcal polysaccharide serotype 3, 14, or 18C (20 µg/ml;American Type Culture Collection, Manassas, Va.). Preliminarykinetic studies revealed that optimal mRNA expression of CD40L,IL-4, IL-12p40, and IFN- $gamma$ was observed at 4 to 6 after stimulation.For comparison purposes, equal numbers of cells were used forboth pre- and postimmunization samples; all cultures were incubatedfor 5 h. After incubation, cells were washed twice with ice-coldphosphate-buffered saline and mRNA wasextracted.

mRNA capture. mRNA was extracted from stimulated cells using the commercial mRNA Capture Kit (Roche, Indianapolis, Ind.) according to themanufacturer's instructions. Briefly, the cell pellet was lysedwith 200 µl of cell lysis buffer; DNA was sheared mechanicallyby passing the lysate through a 21-gauge needle six times. Fourmicroliters of biotin-labeled oligo(dT₂₀) (1:20 dilution fromstock solution) was added to the cell lysate and incubated at37°C for 5 min. After hybridization of the mRNA with biotin-oligo(dT₂₀),50 µl of the solution was added to streptavidin-coated PCR tubesand incubated at 37°C for 3 min. The tubes were then washed threetimes with 250 µl of washingbuffer.

RT-PCR. Captured mRNA was used as substrate for the synthesis of cDNA by reverse transcription (RT). The RT reaction was performedusing avian myeloblastis virus reverse transcriptase (Roche).The reaction was performed at 42°C for 120 min. The cDNA was thenamplified using commercially available sequence specific primersfor IL-4 (456 bp), IL-12p40 (373 bp), IFN- $gamma$ (501 bp), CD40L (293bp), and glyceraldehyde-3-phosphate dehydrogenase (GAPDH) (600bp) (Stratagene, La Jolla, Calif.) by PCR. Direct incorporationof digoxigenin (DIG)-labeled nucleotides in the PCR mixture containing0.2 mM dATP, dCTP, dGTP, 0.19 mM dTTP, and 0.01 mM DIG 11-dUTP(Roche) was used to measure the PCR product by enzyme-linked immunosorbentassay (ELISA). Cycling parameters were as follows: a 5-min denaturationat 95°C and 5-min annealing at 60°C, followed by the appropriatenumber of cycles of 1 min at 72°C, 45 s at 95°C, 45 s at 60°C,and a final 7 min at 72°C (Twin Block System, Ericomp, San Diego,Calif.). All PCR products were analyzed in preliminary studieswithin the linear range of amplification as follows: IL-4, 34cycles; IL-12p40, 30 cycles; CD40L, 26 cycles; IFN- $gamma$ , 22 cycles,and GAPDH, 18 cycles. In all cases, the resultant PCR productsof 600 bp (GAPDH), 501 bp (IFN- $gamma$ ), 456 bp (IL-4), 373 bp (IL-12p40),and 293 bp (CD40L) were visualized by ethidium bromide stainingon 2% agarose gels under UVlight.

Quantification of PCR amplicons by capillary electrophoresis. Capillary electrophoresis using the Gold-P/ACE System 5000 with laser-induced fluorescence detection (Beckman, Fullerton,Calif.) was performed as previously described (33). To quantifymRNA, the amount of each different amplicon in each PCR samplewas measured by integrating the fluorescence peakareas.

Quantification of PCR amplicons by ELISA-PCR. A commercial ELISA-PCR system (Roche) was used for the semiquantitative detection of DIG-labeled PCR products by a hybridization-basedmicrotiter plate assay. Wells of a streptavidin-coated microtiterplate were filled with 10 µl of PCR product, followed by denaturationwith 25 µl of 0.2 N NaOH for 5 min and hybridization with 2 pmolof the respective 3'-biotinylated capture probe (Integrated DNATechnologies, Coralville, Iowa). The capture probes were specificfor the following amplified target sequences: 5'-GAC AAC TTT GGTATC GTG GAA GGA-3' for GAPDH, 5'GGC ATT TTG AAG AAT TGG AAA GAGGAG-3' for IFN- $gamma$ , 5'-TGC GTT CAG GTC CAG GGC AAG AGC-3' for IL-12p40,5'-TTC ACA GGA CAG GAA TTC AAG CCC-3' for IL-4, and 5'-AAT CCATTC ACT TGG GAG GAG-3' for CD40L. Capture was allowed to proceedfor 3 h at 45°C. Afterwards, the wells were washed three timeswith washing solution (Roche). To each well was added 200 µl ofanti-DIG-peroxidase (10 U/ml; Roche) diluted 1:1,000 in a buffercontaining 100 mM Tris-HCl and 150 mM NaCl (pH 7.5). The plateswere incubated at 37°C for 30 min and then washed as before. Thereaction was visualized by adding 200 µl of ABTS [2,2'-azinobis(3-ethylbenzthiazdinesulfonicacid)] substrate solution (Roche) to each well and incubatingthe plates at 37°C for 30 min in the dark. The optical density(OD) was read at 405 nm with a reference at 490 nm using a Bio-Rad(Hercules, Calif.) reader. The run was considered valid if allnegative control values were less than 0.2 OD unit and the positivecontrol value was greater than 1.0 OD unit. ODs were convertedinto logs of copy numbers of initial cDNAs in the patient samples.Quantification of PCR products was performed by comparison toa standard curve. The standard curve for each amplicon was createdusing serial dilutions of known concentrations (logs of copy numbersof initial cDNAs) of plasmids coding for GAPDH, IFN- $gamma$ , IL-12p40,IL-4, or CD40L (American Type Culture Collection). Plasmids wereisolated, serially diluted, PCR amplified, and detected as describedabove. OD units for patient samples were then converted to copynumbers based on their respective standardcurves.

ELISA for antipneumococcal IgG. IgG antipneumococcal antibody levels against serotypes 1, 3, 4, 6B, 9V, 14, 18C, 19F, and 23F were determined by an ELISAprotocol calibrated against the FDA 89-SF reference sample (CBER;FDA, Washington, D.C.) as previously described (29).

Statistical analysis. Comparisons between pre- and postimmunization paired data were performed using the Wilcoxon test (one tailed). A P value of<0.05 was consideredsignificant.

	RESULTS

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The geometric means of IgG antibody concentrations specific to pneumococcal polysaccharide serotypes 3, 14, and 18C beforeand 4 to 6 weeks after immunization with 23-PV are shown in Table1. Significant differences in antibody concentrations betweenpre- and postimmunization samples were observed for each serotypestudied. One patient, who failed to respond to the polysaccharidevaccine, showed an adequate response, according to published criteria(28), 4 weeks after immunization with an experimental heptavalentpneumococcal conjugate vaccine (data not shown). Nonimmunizedcontrols showed no increase in antibody concentrations from onesample to the other (data not shown).

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TABLE 1. Geometric mean concentrations of IgG antibodies against pneumococcal polysaccharides in 14 children immunized with the 23-PV

A representative agarose gel with pre- and postimmunization samples from a patient who had a significant antibody responseto 23-PV shows the ethidium bromide-stained PCR products fromboth unstimulated cells and cells stimulated (Fig. 1). GAPDH mRNA,the product of a housekeeping gene used as control, can be visualizedas a 600-bp band showing the same level of intensity in everylane. In contrast, no CD40L or cytokine message was detected inunstimulated cultures. In pre- and postimmunization samples, ConAstimulated detectable mRNA expression of CD40L, IFN- $gamma$ , IL-4, andIL-12p40, while TT induced some mRNA expression of IFN- $gamma$ but weakexpression of IL-4 and IL-12p40. All pneumococcal antigens induceddetectable IL-4 mRNA levels in postimmunization samples and CD40LmRNA levels in pre- and, even more intensively, postimmunizationsamples. These initial observations led us to use more sensitivemethods to quantify the PCR products in order to test the possibilitythat pneumococcal immunization may up-regulate CD40L and IL-4expression.

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FIG. 1. Agarose gel electrophoresis of RT-PCR products. Lanes show RT-PCR products from preimmunization (lanes 1) and postimmunization (lanes 2) samples unstimulated (Uns) or stimulated for 5 h with the optimal concentration of ConA, TT, 23-PV, or serotype (Ser) 3, 14, or 18C. The sizes of the RT-PCR products were compared to those of DNA fragments of the markers.

The initial PCR results visualized by ethidium bromide staining for one patient were confirmed in the entire study population.The amount of PCR product in each sample was initially measuredby two different methods: capillary electrophoresis and ELISA-PCR.Both methods are semiquantitative and generated comparable results.Here we present results obtained with ELISA-PCR.

Unstimulated cells from pre- and postimmunization samples produced small amounts of CD40L mRNA expression. In ConA- and antigen-stimulatedcultures, CD40L mRNA expression increased over that of unstimulatedcultures in both pre- and postimmunization samples. The intensityof CD40L message induced by the individual polysaccharide serotypes3, 14, and 18C was significantly higher (P < 0.05) in post- thanin preimmunization samples (Fig. 2A). The response to 23-PV wasalso increased, but the difference did not reach statistical significance.

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FIG. 2. mRNA expression of CD40L and cytokines in PBMC before and 4 to 6 weeks after immunization with 23-PV in unstimulated cells (Uns) or in cells stimulated for 5 h with the optimal concentration of ConA, TT, 23-PV, or serotype (Ser) 3, 14, or 18C. RT-PCR products were quantified by ELISA-PCR as described in Materials and Methods. Results are expressed as the geometric mean (GM) of the logs of copy numbers in pre- and post-immunization samples (*, P < 0.05).

Analysis of the cytokine profiles induced in vitro in these patients shows differences in the intensity of mRNA expressionfor different stimuli. ConA induced higher expression of IL-4,IFN- $gamma$ , and IL-12p40 mRNAs in pre- and postimmunization samplesin comparison to unstimulated cells (Fig. 2B to D). Similarly,the intensity of mRNA expression induced by TT was significantlyhigher than that of unstimulated cells for IL-4 and IL-12p40.There was no change in IFN- $gamma$ mRNA from pre- to postimmunizationin unstimulated and stimulated samples (Fig. 2C). Pneumococcalpolysaccharide antigens induced higher mRNA expression of IL-4,but not IFN- $gamma$ or IL-12p40, mRNA compared to unstimulated cultures.The differences in intensity of IL-4 mRNA expression between pre-and postimmunization samples were significant (P < 0.05) in cellsstimulated with the individual serotypes 3, 14, and 18C (Fig.2B). The response to 23-PV was also increased, but the differencedid not reach statistical significance. mRNAs for CD40L and cytokinesdid not change in the control group (data notshown).

The individual responses shown in Fig. 3 and 4 demonstrate that cells stimulated with pneumococcal serotypes 3, 14, and 18Chad significantly increased (P < 0.05) CD40L and IL-4 mRNA expressionin post-compared to preimmunization samples. These increases werepresent in all of the patients studied. In contrast, no significantchanges in the level of CD40L or IL-4 mRNA expression were observedin the control group.

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FIG. 3. mRNA expression of CD40L in PBMC cultures from 14 patients before and 4 to 6 weeks after immunization with 23-PV compared to mRNA expression in PBMC cultures from four unimmunized controls. Several patient values are very similar, so some lines are superimposed. Cells were stimulated for 5 h with the optimal concentration of pneumococcal polysaccharide serotype 3, 14 or 18C. ELISA-PCR results are expressed as copy numbers.

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FIG. 4. mRNA expression of IL-4 in PBMC cultures from 14 patients before and 4 to 6 weeks after immunization with 23-PV compared to mRNA expression in PBMC cultures from 4 unimmunized controls. Several patient values are very similar, so some lines are superimposed. Cells were stimulated for 5 h with the optimal concentration of pneumococcal polysaccharide serotype 3, 14, or 18C. ELISA-PCR results are expressed as copy numbers.

The intensity of mRNA expression of CD40L and cytokines was studied in preimmunization, post-23-PV, and postconjugate samplesfrom a patient who received the pneumococcal conjugate vaccineafter failing to respond to 23-PV. Higher levels of mRNA expressionof CD40L and IL-4 were observed in ConA- and TT-stimulated culturesfrom postconjugate samples in comparison to pre- or post-23-PVsamples (Fig. 5, top panel). Cultures stimulated with 23-PV orwith the individual serotypes showed a marked increase in mRNAexpression of CD40L and, more significantly, of IL-4 in postconjugatesamples in comparison to post-23-PV or preimmunization samples(Fig. 5, bottom panel). The conjugate vaccine did not increaseIL-12p40 or IFN- $gamma$ mRNA (data not shown).

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FIG. 5. Relative quantities of CD40L and IL-4 mRNA in PBMC from one patient before and 4 to 6 weeks after immunization with 23-PV and 4 weeks after a second immunization with the 7-valent pneumococcal conjugate vaccine (PC). mRNA was quantified by RT-PCR and capillary electrophoresis. Results are expressed as the ratio of the peak area of subunit mRNA to that of the mRNA of the housekeeping gene for GAPDH. Ser, serotype.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Our observation that CD40L mRNA expression in PBMC is increased in vitro by polysaccharide antigens is consistent with theobservation that TI-2 antigens induce CD40L expression in vivo(32). CD40L is expressed on activated CD4⁺ T cells, monocytes, B cells, and NK cells (7). The small bloodsample that we could obtain from children precluded separationand identification of different cell types or measurement of cytokinesecretion in our study. However, since T cells are the largestproportion of cells in the PBMC preparations used in our studies,our results are suggestive of T-cell activation by polysaccharideantigens. This is also supported by the observation of a significantincrease in IL-4 mRNA in response to stimulation with pneumococcalpolysaccharide antigens. On the other hand, the lack of IL-12stimulation by pneumococcal polysaccharides suggests that monocytes,another possible source of CD40L, are not major contributors tothe observed increase in CD40L mRNA (4, 12).

A role for NK cells in the increase of CD40L and IL-4 mRNAs observed in our experiments cannot be ruled out. Several reportshave suggested that induction of an antibody response to TI-2antigens does not require the participation of T cells but requirescytokines from cells other than T cells, such as NK cells (13,14, 26, 34). On the other hand, our hypothesis that T cellsdo respond to pneumococcal polysaccharides is in agreement withnumerous studies that have questioned the T-cell independenceof the response to TI-2 antigens (10, 13-15, 21, 31). Studiesusing flow cytometric methods to identify the cells expressingcytokines in cultures stimulated with pneumococcal polysaccharideantigens are in progress in ourlaboratory.

The increase in IL-4 mRNA suggests that pneumococcal polysaccharides induce a Th2 response, characterized by increased secretionof IL-4, which shifts the immune response to IgG and IgE antibodyproduction (16, 17, 22). Our results are in agreement withthe observation of an IL-4 regulation of in vivo antibody productionin response to TI-2 antigens in experimental animals (11). Th1cells do not appear to be involved in the response to pneumococcalpolysaccharides, since neither IL-12 nor IFN- $gamma$ mRNA increasedin our experiments. An increase in these cytokine messages isobserved in Th1 responses, where IL-12 promotes the differentiationof naive T cells to Th1 cells and activation of these cells resultsin IFN- $gamma$ production (12, 25).

Increased CD40L and IL-4 mRNAs in samples obtained 4 weeks after immunization confirm the same observations made prior toimmunization. These results suggest that pneumococcal polysaccharideimmunization may produce an expansion of memory T cells that persistsfor several weeks after immunization. The specificity of thisresponse to pneumococcal antigens was supported by the contrastingresults observed in cultures stimulated with ConA, a nonspecificstimulator, or with TT, a recall protein antigen, which induceda similar increase in CD40L and IL-4 mRNAs in pre- and postimmunizationsamples. These observation suggest that the in vitro responseto TT was a secondary response in patients, who had all been immunizedwith vaccines containing TT in the past. The lack of significantdifferences in CD40L or IL-4 mRNA expression between two separatesamples in the unimmunized control group further supports theidea that observed differences in pre- and postimmunization sampleswere due to an immune response to pneumococcal polysaccharidesinvivo.

Our observation for one patient who failed to mount an adequate antibody response to the pneumococcal polysaccharide vaccineis of interest. This patient showed a significant increase inantibodies to serotypes 3, 14, and 18C after vaccination withthe CRM197 pneumococcal conjugate vaccine (28). Immunizationwith this conjugate vaccine induced not only greater expressionof CD40L and IL-4 mRNAs in response to specific stimulation withpneumococcal polysaccharide antigens but also an increase in mRNAexpression in response to ConA and TT. If similar observationscan be confirmed for a larger number of individuals, it may reflectthe adjuvant effect of the carrier protein in the conjugatevaccine.

The immune response to allergens has been shown to be a Th2 response, and allergen immunotherapy is thought to shift Th2-type to Th1-type responses (24). Now that the pneumococcal conjugatevaccine is available and has been recommended for generalizeduse in infants at 2, 4, 6, and 12 to 15 months of age, it willbe important to study the effect of this vaccine on the Th1-Th2balance in large numbers ofindividuals.

In summary, this study shows that pneumococcal polysaccharide antigens induce the expression of CD40L and a Th2 response andthat these responses are up-regulated by immunization with pneumococcalvaccines paralleling the increase in circulating IgG antipneumococcalantibody concentrations. Further studies aimed at identifyingthe cells regulating the response to pneumococcal polysaccharideantigens and investigating the role of pneumococcal immunizationin the Th1-Th2 balance should expand the observations reportedhere.

	ACKNOWLEDGMENTS

This research was supported in part by an unrestricted grant from Wyeth-Lederle.

We thank Patricia A. Giangrosso for editorial assistance in the preparation of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Pediatrics, LSU Health Sciences Center, 1542 Tulane Ave. New Orleans,LA 70112-2822. Phone: (504) 568-8176. Fax: (504) 568-7598. E-mail:lleiva{at}lsuhsc.edu.

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Abstract
Introduction
Materials and Methods
Results
Discussion
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20. Pecanha, L. M. T., C. M. Snapper, F. D. Finkelman, and J. J. Mond. 1991. Dextran-conjugated anti-Ig antibodies as a model for T-cell independent type 2 antigen-mediated stimulation of Ig secretion in vitro. I. Lymphokine dependence. J. Immunol. 146:833-839[Abstract].

21. Pecanha, L. M. T., C. M. Snapper, A. Lees, and J. J. Mond. 1992. Lymphokine control of type 2 antigen response. IL-10 inhibits IL-5 but not IL-2-induced Ig secretion by T cell-independent antigens. J. Immunol. 148:3427-3432[Abstract].

22. Romagnani, S. 1994. Lymphokine production by human T cells in disease states. Annu. Rev Immunol 12:227-257[CrossRef][Medline].

23. Sanders, L. A., G. T. Rijkers, W. Kuis, A. J. Tenbergen-Meekes, B. R. de Graeff-Meeder, I. Hiemstra, and B. J. Zegers. 1993. Defective antipneumococcal polysaccharide antibody response in children with recurrent respiratory tract infections. J. Allergy Clin. Immunol. 91:110-119[CrossRef][Medline].

24. Secrist, H., C. J. Chelen, Y. Wen, J. D. Marshall, and D. T. Umetsu. 1993. Allergen immunotherapy decreases interleukin 4 production in CD4+ T cells from allergic individuals. J. Exp. Med. 178:2123-2130[Abstract/Free Full Text].

25. Seder, R. A., and E. Paul. 1994. Acquisition of lymphokine-producing phenotype by CD4+ T cells. Annu. Rev. Immunol. 12:635-655[CrossRef][Medline].

26. Snapper, C. M., H. Yamaguchi, M. A. Moorman, and J. J. Mond. 1994. An in vitro model for T cell-independent induction of humoral immunity. A requirement for NK cells. J. Immunol. 152:4884-4892[Abstract].

27. Sniadak, D. H., B. Schwartz, H. Lipman, J. Bogaerts, J. C. Butler, R. Dagan, G. Echaniz-Aviles, N. Lloyd-Evans, A. Fenoli, N. I. Girgis, J. Henrichsen, K. Klugman, D. Lehmann, A. K. Takala, J. Vandepitte, S. Gove, and R. F. Breiman. 1995. Potential interventions for the prevention of childhood pneumonia: geographic and temporal differences in serotype and serogroup distribution of sterile site pneumococcal isolates from children $---$ implications for vaccine strategies. Pediatr. Infect. Dis. J. 14:503-510[Medline].

28. Sorensen, R. U., L. E. Leiva, P. A. Giangrosso, B. Butler, D. M. Sacerdote, N. Bradford, and C. Moore. 1998. Response to a heptavalent conjugate Streptococcus pneumoniae vaccine in children with recurrent infections who are unresponsive to the polyssaccharide vaccine. Pediatr. Infect. Dis. J. 17:685-691[CrossRef][Medline].

29. Sorensen, R. U., L. E. Leiva, F. C. Javier, D. M. Sacerdote, N. Bradford, B. Butler, P. Giangrosso, and C. Moore. 1998. Influence of age on the response to Streptococcus pneumoniae vaccine in patients with recurrent infections and normal immunoglobulin concentrations. J. Allergy Clin. Immunol. 102:215-221[CrossRef][Medline].

30. Sorensen, R. U., and C. Moore. 1994. Immunology in the pediatrician's office. Pediatr. Clin. N. Am. 41:691-714[Medline].

31. Van Den Eertwegh, A. J. M., M. J. Fasbender, M. M. Schellekens, A. V. Oudenaren, W. J. A. Boersma, and E. Claassen. 1991. In vivo kinetics and characterization of IFN- $gamma$ producing cells during a thymus-independent immune response. J. Immunol. 147:439-446[Abstract].

32. Van den Eertwegh, A. J. M., R. J. Noelle, M. Roy, D. M. Sheperd, A. Aruffo, J. A. Ledbetter, W. J. A. Boersma, and E. Claasen. 1993. In vivo CD40-gp39 interactions are essential for thymus-dependent immunity. I. CD40-gp39 interactions are essential for thymus-dependent humoral immunity and identify sites of cognate interactions in vivo. J. Exp. Med. 178:1555-1565[Abstract/Free Full Text].

33. Vehaskari, V. M., J. M. Hempe, J. Manning, D. H. Aviles, and M. C. Carmichael. 1998. Developmental regulation of ENaC subunit mRNA levels in rat kidney. Am. J. Physiol. 274:C1661-C1666.

34. Wilder, J. A., C. Y. Koh, and D. Yuan. 1996. The role of NK cells during in vivo antigen-specific antibody responses. J. Immunol. 156:146-152[Abstract].

35. Zora, J. A., H. J. Silk, and D. G. Tinkelman. 1993. Evaluation of postimmunization pneumococcal titers in children with recurrent infections and normal levels of immunoglobulin. Ann. Allergy 70:283-287[Medline].

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Sen, G., Khan, A. Q., Chen, Q., Snapper, C. M. (2005). In Vivo Humoral Immune Responses to Isolated Pneumococcal Polysaccharides Are Dependent on the Presence of Associated TLR Ligands. J. Immunol. 175: 3084-3091 [Abstract] [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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13.	Mond, J. J., A. Lees, and C. M. Snapper. 1995. T cell-independent antigens type 2. Annu. Rev. Immunol. 13:655-692[CrossRef][Medline].
14.	Mond, J. J., Q. Vos, A. Lees, and C. M. Snapper. 1995. T cell independent antigens. Curr. Opin. Immunol. 7:349-354[CrossRef][Medline].
15.	Mongini, P. K., K. E. Stein, and W. E. Paul. 1981. T cell regulation of IgG subclass antibody production in response to T-independent antigens. J. Exp. Med. 153:1-12[Abstract/Free Full Text].
16.	Mosmann, T. R., and S. Sad. 1996. The expanding universe of T-cell subsets: Th1, Th2 and more. Immunol. Today 17:139-146.
17.	Nakamura, T., Y. Kamogawa, K. Bottomly, and R. A. Flavell. 1997. Polarization of IL-4 and IFN- $gamma$ -producing CD4⁺ T cells following activation of naive CD4⁺ T cells. J. Immunol. 158:1085-1094[Abstract].
18.	Nishioka, Y., and P. E. Lipsky. 1994. The role of CD40-CD40 ligand interaction in human T cell-B cell collaboration. J. Immunol. 153:1027-1036[Abstract].
19.	Noelle, R. J., M. Roy, D. M. Shepherd, I. Stamenkovic, J. A. Ledbetter, and A. Arufo. 1992. A 39-kDa protein on activated helper T cells binds CD40 and transduces the signal for cognate activation of B cells. Proc. Natl. Acad. Sci. USA 89:6550-6554[Abstract/Free Full Text].
20.	Pecanha, L. M. T., C. M. Snapper, F. D. Finkelman, and J. J. Mond. 1991. Dextran-conjugated anti-Ig antibodies as a model for T-cell independent type 2 antigen-mediated stimulation of Ig secretion in vitro. I. Lymphokine dependence. J. Immunol. 146:833-839[Abstract].
21.	Pecanha, L. M. T., C. M. Snapper, A. Lees, and J. J. Mond. 1992. Lymphokine control of type 2 antigen response. IL-10 inhibits IL-5 but not IL-2-induced Ig secretion by T cell-independent antigens. J. Immunol. 148:3427-3432[Abstract].
22.	Romagnani, S. 1994. Lymphokine production by human T cells in disease states. Annu. Rev Immunol 12:227-257[CrossRef][Medline].
23.	Sanders, L. A., G. T. Rijkers, W. Kuis, A. J. Tenbergen-Meekes, B. R. de Graeff-Meeder, I. Hiemstra, and B. J. Zegers. 1993. Defective antipneumococcal polysaccharide antibody response in children with recurrent respiratory tract infections. J. Allergy Clin. Immunol. 91:110-119[CrossRef][Medline].
24.	Secrist, H., C. J. Chelen, Y. Wen, J. D. Marshall, and D. T. Umetsu. 1993. Allergen immunotherapy decreases interleukin 4 production in CD4+ T cells from allergic individuals. J. Exp. Med. 178:2123-2130[Abstract/Free Full Text].
25.	Seder, R. A., and E. Paul. 1994. Acquisition of lymphokine-producing phenotype by CD4+ T cells. Annu. Rev. Immunol. 12:635-655[CrossRef][Medline].
26.	Snapper, C. M., H. Yamaguchi, M. A. Moorman, and J. J. Mond. 1994. An in vitro model for T cell-independent induction of humoral immunity. A requirement for NK cells. J. Immunol. 152:4884-4892[Abstract].
27.	Sniadak, D. H., B. Schwartz, H. Lipman, J. Bogaerts, J. C. Butler, R. Dagan, G. Echaniz-Aviles, N. Lloyd-Evans, A. Fenoli, N. I. Girgis, J. Henrichsen, K. Klugman, D. Lehmann, A. K. Takala, J. Vandepitte, S. Gove, and R. F. Breiman. 1995. Potential interventions for the prevention of childhood pneumonia: geographic and temporal differences in serotype and serogroup distribution of sterile site pneumococcal isolates from children $---$ implications for vaccine strategies. Pediatr. Infect. Dis. J. 14:503-510[Medline].
28.	Sorensen, R. U., L. E. Leiva, P. A. Giangrosso, B. Butler, D. M. Sacerdote, N. Bradford, and C. Moore. 1998. Response to a heptavalent conjugate Streptococcus pneumoniae vaccine in children with recurrent infections who are unresponsive to the polyssaccharide vaccine. Pediatr. Infect. Dis. J. 17:685-691[CrossRef][Medline].
29.	Sorensen, R. U., L. E. Leiva, F. C. Javier, D. M. Sacerdote, N. Bradford, B. Butler, P. Giangrosso, and C. Moore. 1998. Influence of age on the response to Streptococcus pneumoniae vaccine in patients with recurrent infections and normal immunoglobulin concentrations. J. Allergy Clin. Immunol. 102:215-221[CrossRef][Medline].
30.	Sorensen, R. U., and C. Moore. 1994. Immunology in the pediatrician's office. Pediatr. Clin. N. Am. 41:691-714[Medline].
31.	Van Den Eertwegh, A. J. M., M. J. Fasbender, M. M. Schellekens, A. V. Oudenaren, W. J. A. Boersma, and E. Claassen. 1991. In vivo kinetics and characterization of IFN- $gamma$ producing cells during a thymus-independent immune response. J. Immunol. 147:439-446[Abstract].
32.	Van den Eertwegh, A. J. M., R. J. Noelle, M. Roy, D. M. Sheperd, A. Aruffo, J. A. Ledbetter, W. J. A. Boersma, and E. Claasen. 1993. In vivo CD40-gp39 interactions are essential for thymus-dependent immunity. I. CD40-gp39 interactions are essential for thymus-dependent humoral immunity and identify sites of cognate interactions in vivo. J. Exp. Med. 178:1555-1565[Abstract/Free Full Text].
33.	Vehaskari, V. M., J. M. Hempe, J. Manning, D. H. Aviles, and M. C. Carmichael. 1998. Developmental regulation of ENaC subunit mRNA levels in rat kidney. Am. J. Physiol. 274:C1661-C1666.
34.	Wilder, J. A., C. Y. Koh, and D. Yuan. 1996. The role of NK cells during in vivo antigen-specific antibody responses. J. Immunol. 156:146-152[Abstract].
35.	Zora, J. A., H. J. Silk, and D. G. Tinkelman. 1993. Evaluation of postimmunization pneumococcal titers in children with recurrent infections and normal levels of immunoglobulin. Ann. Allergy 70:283-287[Medline].