Invariant V{alpha}14 Chain NKT Cells Promote Plasmodium berghei Circumsporozoite Protein-Specific Gamma Interferon- and Tumor Necrosis Factor Alpha-Producing CD8+ T Cells in the Liver after Poxvirus Vaccination of Mice

Understanding the protective mechanism in the liver inducedby recombinant vaccines against the pre-erythrocytic stagesof malaria is important for vaccine development. Most studiesin mice have focused on splenic and peripheral blood T cellsand identified gamma interferon (IFN- ${gamma}$ )-producing CD8⁺ T cellsas correlates of protection, which can be induced by prime-boostvaccination with recombinant poxviruses. Invariant natural killerT (V ${alpha}$ 14iNKT) cells can also protect against liver stage malaria,when activated, and are abundant in the liver. Since poxviruseshave nonspecific immunomodulating effects, which are incompletelyunderstood, we investigated whether recombinant poxviruses affectthe protective properties of hepatic V ${alpha}$ 14iNKT cells and thusvaccine efficacy. We show that intradermal vaccination withrecombinant poxviruses activated V ${alpha}$ 14iNKT cells and NK cellsin the livers of BALB/c mice while inducing IFN- ${gamma}$ - and tumornecrosis factor alpha (TNF- ${alpha}$ )-producing pre-erythrocytic stageantigen-specific CD8⁺ T cells. Greater numbers of hepatic V ${alpha}$ 14iNKTcells secreted interleukin-4 than IFN- ${gamma}$ . Vaccinated V ${alpha}$ 14iNKT-cell-deficientmice had lower, but still protective levels of hepatic and splenicIFN- ${gamma}$ ⁺ and TNF- ${alpha}$ ⁺ CD8⁺ T cells and better protection rates laterafter challenge with Plasmodium berghei sporozoites. Therefore,vaccine-activated hepatic V ${alpha}$ 14iNKT cells help in generating specificT cells but are not required for protection induced by recombinantpoxviruses. Furthermore, double-positive INF- ${gamma}$ ⁺/TNF- ${alpha}$ ⁺ CD8⁺ Tcells were enriched in protected livers, suggesting that cellsexpressing both of these cytokines may be most relevant forprotection.

INTRODUCTION

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Introduction

The malaria parasites, Plasmodium spp., are a leading causeof death and morbidity in tropical countries. In the face ofthe increasing drug resistance of these parasites, other effectiveinterventions, such as vaccines, that target the pre-erythrocyticliver, blood, and transmission stages are urgently needed (33).Understanding the protective immune mechanisms in the livermay be crucial for the development of a pre-erythrocytic stagevaccine (14). Natural and vaccine-induced immunity to liver-stagemalaria requires specific and vigorous cellular immunity mediatedby gamma interferon (IFN- ${gamma}$ ), as well as nonspecific interleukin-12(IL-12), IFN- ${gamma}$ -producing natural killer (NK) cells, and ${gamma}$ ${delta}$ T cells(13, 14, 20, 42, 43). The best-defined and clinically appliedcorrelates of protection are IFN- ${gamma}$ -producing pre-erythrocyticstage-specific CD4⁺ and CD8⁺ T cells, which trigger the intracellularnitric oxide pathway in hepatocytes infected by sporozoites(20, 43). Infection with radiation-attenuated sporozoites inducessuch protective T-cell responses, as does heterologous prime-boostimmunization with recombinant DNA and viral vectors, encodingpre-erythrocytic-stage antigens, such as the circumsporozoiteprotein (CSP), a major sporozoite surface antigen (15, 43, 45).Attenuated recombinant poxviruses such as modified vacciniavirus Ankara (MVA) (32, 45) and the new fowlpox strain, FP9(3), have been successfully used for heterologous T-cell boostingand confer substantial protection against malaria in animals,as well as in some volunteers in phase IIa clinical trials (3;unpublished data).

Vaccine-induced T-lymphocyte responses have mainly been describedin peripheral blood and murine spleens but not in the liver,except for studies on sporozoite immunization (4, 28). Sincethe immunogenic properties of attenuated recombinant poxvirusesare incompletely understood, we examined the influence of FP9and MVA vaccination on liver lymphocytes in more detail aftera recent study demonstrating the induction of hepatic IFN- ${gamma}$ -producingCD8⁺ T cells by these vaccines (3).

We investigated whether poxvirus vaccination induced not onlyIFN- ${gamma}$ -producing, but also TNF- ${alpha}$ -producing CD8⁺ T cells in themurine liver and whether they correlated with protection againstsporozoite challenge. The induction of TNF- ${alpha}$ -producing T cellsis of particular interest in malaria because TNF- ${alpha}$ can inhibitboth liver- and blood-stage parasites (23, 24, 29, 36) and synergizeswith IFN- ${gamma}$ to induce nitric oxide and kill parasites (23, 24).

In addition to CSP-specific CD8⁺ T cells, we also examined nonspecificinvariant natural killer T (V ${alpha}$ 14iNKT) and NK cells, since littleis known about the paraspecific effects of attenuated poxviruses(31). It is known from live or killed viruses that they canactivate peripheral blood, splenic, and hepatic NK cells (12,31, 41). V ${alpha}$ 14iNKT cells are a CD4⁺ or CD4^– CD8^– NKcell receptor bearing subpopulation of T cells with restrictedT-cell-receptor (TCR) repertoire expression. In mice this includesthe invariant V ${alpha}$ 14-J ${alpha}$ 18/Vß2/Vß7/Vß8.2chains. V ${alpha}$ 14iNKT cells are particularly abundant in the murineliver and can be rapidly activated similar to NK cells (10,16). In contrast to NK cells, they can produce not only IFN- ${gamma}$ but also IL-4 and thus can promote Th1 or Th2 type-specificimmunity, activating antigen-presenting cells, NK cells, B cells,and T cells (7, 10, 16, 42). Since the liver is also known tobe a Th2-driving environment, which could hamper vaccine-inducedTh1 immunity against liver-stage parasites (10, 28), we havestudied here IL-4 and IFN- ${gamma}$ production by V ${alpha}$ 14iNKT cells. IL-4,derived from conventional CD4⁺ T cells, can promote the generationof liver-stage-specific CD8⁺ T cells (8) but also suppress Th1immunity (49). V ${alpha}$ 14iNKT cells release cytokines upon TCR-mediatedrecognition of the synthetic glycolipid ligand alpha-galactosylceramide( ${alpha}$ -GalCer), which binds to CD1d molecules on antigen-presentingcells (26). Triggered by ${alpha}$ -GalCer, IFN- ${gamma}$ -producing V ${alpha}$ 14iNKT cellsconfer very short-term protection and adjuvant vaccine-inducedIFN- ${gamma}$ -producing specific T cells against murine liver-stage malaria(18, 19). We hypothesized that there might be a synergisticinduction of V ${alpha}$ 14iNKT, CD8⁺ T, and NK cells by poxvirus vaccinationindependently from ${alpha}$ -GalCer and that this might influence protection.To test our hypotheses, we immunized wild-type (WT) BALB/c miceand V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18-chain knockout (KO; J ${alpha}$ 18^–/–)mice with malaria poxvirus vaccines and challenged them withinfectious sporozoites.

This comparative analysis of hepatic and splenic antigen-specificCD8⁺ T cells, V ${alpha}$ 14iNKT cells, and NK cells after malaria poxvirusvaccination and challenge provides novel information on liverimmunity against pre-erythrocytic-stage malaria.

MATERIALS AND METHODS

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Materials and Methods

Immunization of mice with malaria vaccines. We used 6- to 12-week-old female WT BALB/c mice and J ${alpha}$ 18^–/–mice (formerly J ${alpha}$ 281^–/–, backcrossed more than 10times to BALB/c background) (mainly female) mice, which lackV ${alpha}$ 14iNKT cells, in these experiments. Mice were originally obtainedfrom The Jackson Laboratory (Bar Harbor, Maine) and Chiba University(Chuoku, Chiba, Japan) (11) and were bred at the Oxford Universityanimal facilities under specific-pathogen-free conditions. Themice were handled according to the Home Office Animals Act 1986(Scientific Procedures) guidelines under project license PPL30/1805. Construction of the MVAPbCSP vaccine encoding the P.berghei circumsporozoite protein (PbCSP) has been previouslydescribed (45). The attenuated fowlpox vaccine strain FP9 wasproduced by multiple passage of WT strain HP-1 as previouslydescribed (3, 30). For the empty control viruses (FP9/MVAlacZ),fowlpox vaccine strains were recombined with pEFL29 withoutan inserted antigen but contain the ß-galactosidasegene under a late promoter (3). Recombinant viruses were administeredintradermally bilaterally into the ears at a dose of 10⁶ PFU,diluted in 50 µl of endotoxin-free Dulbecco’s phosphate-bufferedsaline (PBS; Sigma). Mice were primed with FP9PbCSP (F) andboosted 2 weeks later with MVAPbCSP (M). Some mice were prime-boostedwith the control viruses FP9lacZ and MVAlacZ. Mice were sacrificedfor immunogenicity assays 14 to 40 days postimmunization.

Challenge of mice with P. berghei sporozoites. Laboratory-reared female Anopheles stephensi mosquitoes infectedwith P. berghei sporozoites (ANKA strain clone 234) were maintainedat 21°C for 21 to 25 days after feeding on infected mice.Mosquito salivary glands were dissected and homogenized in 4°CRPMI 1640 media (Sigma) to release sporozoites (45). Groupsof F/M-vaccinated mice (n = 3 to 17) were challenged and, ascontrols, naive mice (n = 3 to 9) were infected with 1,000 sporozoites(100 µl) by intravenous injection into the lateral tailvein, providing a stringent challenge (3). Blood-stage infection(patency) was monitored from days 3 to 13 postinfection or challengefor the presence of ring forms by using Giemsa-stained bloodsmears. Mice were either sacrificed 1 day or 6 to 13 days afterchallenge or maintained for rechallenge at 40 days after immunization.

Cell preparation. Splenocytes were isolated by mechanical disruption of spleens,filtration, and red blood cell lysis in ammonium chloride bufferand prepared for enzyme-linked immunospot (ELISPOT) assays andfluorescence-activated cell sorter (FACS) analysis as previouslydescribed (45). Only lymphocytes with >98% viability weregated, and absolute numbers were counted on a CASY Cell Analyzer(Model TT; Schaerfe System GmbH, Reutlingen, Germany). For theisolation of hepatic mononuclear cells (MNC), livers were flushedin situ via the portal vein with 10 ml of PBS containing 10%fetal bovine serum. After mechanical disruption and filtration,pelleted cells were resuspended in 5 ml of buffered 80% Percoll(Amersham Pharmacia Biotech; supplemented with 0.5% bicarbonate[7%], 10% 10xRPMI, 1% fetal bovine serum) overlaid with 5 mlof 35% buffered Percoll and spun at room temperature at 500x g without brake for 25 min. MNC from the interface were pelleted,washed, and resuspended in 1 ml of medium, and lymphocytes werecounted as described above and further processed for ELISPOTassays or FACS analysis.

ELISPOT assays. IFN- ${gamma}$ , tumor necrosis factor alpha (TNF- ${alpha}$ ), or IL-4 ex vivo ELISPOTassays on splenocytes and hepatic MNC were conducted as previouslydescribed for splenic IFN- ${gamma}$ -producing T cells (45). Briefly,ELISPOT plates (Millipore) were coated with 10 µg of anti-mouseIFN- ${gamma}$ antibody (Ab; clone R4-6A2), anti-TNF- ${alpha}$ Ab (clone G281-2626),or anti-IL-4 Ab (clone BVD4-1D11)/ml (Becton Dickinson). Targetcells (0.5 x 10⁶ cells/well) were prepared by pulsing naivesplenocytes with (i) the H-2K^d-restricted test peptide Pb9 (SYIPSAEKI),an immunodominant CD8 epitope from P. berghei CSP, which isonly recognized by peptide Pb9-specific CD8⁺ T cells; (ii) ${alpha}$ -GalCer(provided by Kirin Brewery, Ltd., Tokyo, Japan) to detect ${alpha}$ -GalCerresponsive V ${alpha}$ 14iNKT cells; or (iii) an irrelevant control peptide.Splenocytes were applied at 0.5 x 10⁶/well, and liver MNC atvarious cell numbers per milliliter (mean ± the standarddeviation [SD]: [2.5 ± 2] x 10⁶/ml; [1.2 ± 1]x 10⁵/well), and responses as spot-forming cells (SFC) per millionwere calculated from duplicate wells after subtraction of negativecontrol wells. After 18 to 24 h of incubation at 37°C under5% CO₂, the plates were washed once with distilled water andfour times with PBS before overnight incubation with biotinylatedanti-mouse IFN- ${gamma}$ Ab (clone XMG1.2), anti-TNF- ${alpha}$ Ab (clone MP6-XT3),or anti-IL-4 Ab (clone BVD6-24G2) (Becton Dickinson). The assaywas developed by further incubation with streptavidin-alkalinephosphatase polymer (Mabtech; Sigma), and spots were visualizedby adding an alkaline phosphatase substrate solution (Bio-Rad).Spots were counted by using an AID ELISPOT counter (AID GmbH).

Cell staining and FACS analysis. For detection of V ${alpha}$ 14iNKT cells, splenocytes and hepatic MNCwere four-color stained with CD1d/ ${alpha}$ -GalCer tetramer-phycoerythrin(PE), biotinylated anti-TCRß chain Ab (clone H57-597)conjugated with peridinin chlorophyll protein (PerCP), anti-CD8a-allophycocyanin(APC) (Ly-2, clone 53-6.7), and anti-CD4-fluorescein isothiocyanateAb (FITC; clone H129.19) (Becton Dickinson). A total of 15,000to 70,000 gated lymphocytes were acquired. The CD1d/ ${alpha}$ -GalCertetramer was generated by in vitro oxidative refolding chromatographyas previously described (25). NK cells and conventional T cellswere detected by four-color staining with anti-CD49b/Pan-NKcell Ab (clone DX5), biotinylated anti-TCRß chain(clone H57-597) conjugated with streptavidin-PerCP, anti-CD8a-APCAb (Ly-2, clone 53-6.7), and anti-CD4-FITC Ab (clone H129.19).A total of 10,000 lymphocytes were gated at analysis. Intracellularcytokine staining (ICS) was performed on approximately 2 x 10⁶splenocytes and 2 to 8 x 10⁵ liver MNC pooled from two or fourmice, stimulated with peptide Pb9, phytohemagglutinin, or anirrelevant peptide for 6 h. A Cytofix/Cytoperm Plus (with GolgiPlug) kit (Becton Dickinson) was applied according to the manufacturerby using anti-IFN- ${gamma}$ -FITC Ab (clone XMG1.2), biotinylated anti-TNF- ${alpha}$ Ab (clone MP6-XT3) conjugated with streptavidin-PerCP, anti-CD8a-APCAb (clone 53-6.7), and anti-CD3-PE Ab (clone 145-2C11) for staining.Isotype controls were performed with rat immunoglobulin G1 (IgG1)-PE(clone R3-34), rat IgG2a-FITC (clone R35-95), hamster IgG1-FITC(clone A19-3), hamster IgG2 (clone Ha4/8), and rat IgM (cloneR4-22). A total of 30,000 to 200,000 gated lymphocytes wereacquired. The PE-conjugated H-2K^d/Pb9 tetramer was generatedas described previously (2) and applied, together with anti-B220-FITCAb and anti-CD8ß-Tricolor Ab (CalTag-Medsystems),in FACS buffer for incubation of cells for 20 to 30 min at 37°C.All samples were preincubated with Fc-block (anti-FcR ${gamma}$ III/IICD16/CD32 Ab, clone 2.4G2). After staining, all cells were fixedin PBS-2% paraformaldehyde and analyzed by a FACSCalibur instrument(Becton Dickinson) using CellQuest software (Becton Dickinson).

Statistical analysis. The paired-sample and unpaired Student t test was used for analysisof normally distributed data. Differences in protection ratesof P. berghei-infected mice were assessed by using 95% confidenceintervals (CI) according to the method of Newcombe (34, 35).Statistical analysis was performed by using SPSS for Windowsversion 10 (SPSS, Inc.), Microsoft Excel 2001 or, for calculatingthe odds ratio (OR), QuickView 4.0/Statcalc.

RESULTS

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Results

Prime-boost vaccination induces IFN- ${gamma}$ - and TNF- ${alpha}$ -producing pre-erythrocytic-stage antigen-specific CD8⁺ T cells in the liver and spleen. BALB/c mice were intradermally immunized against the P. bergheipre-erythrocytic-stage antigen CSP by heterologous prime-boostpoxvirus vaccination with FP9PbCSP and MVAPbCSP (F/M). First,we determined the total number of CD8⁺ T cells specificallyinduced in the liver and spleen by staining with peptide Pb9-tetramer.About 10% of hepatic CD8⁺ T cells (Fig. 1A) were antigen specific.Next, we analyzed the levels of IFN- ${gamma}$ -producing peptide pb9-specificCD8⁺ T cells in ELISPOT assays. Vaccination clearly inducedequal levels of IFN- ${gamma}$ -producing CD8⁺ T cells in livers (Fig.1B and C) and spleens (Fig. 1D), reaching approximately 1,000SFC/million lymphocytes. Further, we examined in parallel whetherTNF- ${alpha}$ -producing antigen-specific CD8⁺ T cells were generatedalongside IFN- ${gamma}$ -producers, because the total number of peptidePb9-specific tetramer⁺ T cells exceeded that of IFN- ${gamma}$ ⁺/CD8⁺ Tcells alone in ELISPOT assays (for example, 1,000 SFC/millionhepatic lymphocytes corresponds to 0.5 to 1% tetramer⁺ CD8⁺T cells). Vaccination also strongly induced TNF- ${alpha}$ -producing peptidepb9-specific CD8⁺ T cells in livers (Fig. 1B and C) and spleens(Fig. 1D). The TNF- ${alpha}$ secretors exceeded IFN- ${gamma}$ secretors in theliver (ratio of about 2:1) but not in the spleen. The nonspecificbackground production of both cytokines was very low. ICS confirmedthat T cells and not macrophages secreted TNF- ${alpha}$ and thereforeaccounted for the spots observed in ELISPOT assays (data notshown). ICS revealed that vaccination induced double-positive(IFN- ${gamma}$ ⁺/TNF- ${alpha}$ ) CD8⁺ T cells, more in liver than in spleen, uponstimulation with peptide Pb9 (Fig. 1E); ICS isotype controlsshowed no or very little nonspecific staining (Fig. 1F), andcontrols with the irrelevant peptide or phytohemagglutinin werenegative or positive, respectively (data not shown). In addition,in F/M-vaccinated WT mice no IL-4-producing CD8⁺ T cells weredetected by peptide Pb9 ELISPOT assays in the liver or spleenabove low naive background levels (data not shown).

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FIG. 1. Prime-boost vaccination with FP9PbCSP/MVAPbCSP (F/M) induces peptide Pb9-specific IFN- ${gamma}$ -/TNF- ${alpha}$ -producing CD8⁺ T cells, promoted by V ${alpha}$ 14iNKT cells. (A) Representative Pb9 tetramer⁺/CD8⁺-T-cell population (gated first on lymphocytes and then on TCRß⁺ cells) in the liver 14 days after intradermal vaccination of BALB/c mice. The percentages of positive cells in each quadrant are displayed above FACS analysis profiles. (B to D) IFN- ${gamma}$ -producing ( ${blacksquare}$ ) and TNF- ${alpha}$ -producing () peptide Pb9-specific CD8⁺ T cells in the livers (B and C) and spleens (D) of BALB/c WT mice in comparison with V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/– BALB/c mice (n = 4/group). SFC/million lymphocytes (B and D) and total SFC per liver (C) were detected by IFN- ${gamma}$ and TNF- ${alpha}$ ELISPOT assays 20 days after F/M vaccination. Means ± the standard error of the mean (SEM) are shown; the statistical significance was determined by using the Student t test (**, P < 0.01; *, P < 0.05). The results of one representative experiment out of two performed are shown. (E) ICS of CD8⁺/CD3⁺ Pb9-stimulated pooled (n = 2) hepatic lymphocytes and splenocytes from WT mice 40 days after vaccination. The absolute numbers of positive cells per million lymphocytes are shown for the respective quadrants, as calculated from the events (gated on CD8⁺/CD3⁺) for the absolute numbers of CD8⁺ T cells in one million lymphocytes (according gated percentages of CD8⁺ T cells from all lymphocytes) are given below the FACS analysis profiles. (F) ICS isotype control dot plots for IFN- ${gamma}$ /TNF- ${alpha}$ (rat IgG2a) and CD8 (rat IgG1) from hepatic MNC from pooled WT mice 25 days after F/M vaccination (n = 2) and for protected vaccinated WT mice (see Fig. 5D) 9 days after sporozoite challenge, at 40 days postvaccination (n = 2). The percentages of positive cells are shown for the respective quadrants.

V ${alpha}$ 14iNKT cells promote the generation of IFN- ${gamma}$ - and TNF- ${alpha}$ -producing pre-erythrocytic-stage antigen-specific CD8⁺ T cells in the liver and spleen. We determined whether these specific T-cell responses were influencedby the presence of V ${alpha}$ 14iNKT cells in the absence of the activatingligand ${alpha}$ GalCer. F/M vaccination of V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/–mice induced significantly fewer IFN- ${gamma}$ -producing peptide Pb9-specificCD8⁺ T cells in livers and spleens compared to WT mice (Fig.1B to D). In livers, lower frequencies were evident for therelative SFC per million cells (Fig. 1B), as well as for thetotal absolute number per liver (Fig. 1C). This reduction wasalso observed for splenic (Fig. 1D) and particularly stronglyfor hepatic (Fig. 1B and C) TNF- ${alpha}$ -producing CD8⁺ T cells in theabsence of V ${alpha}$ 14iNKT cells. However, taken together, approximately500 and 1,000 SFC/million lymphocytes were still induced inthe liver and spleen, respectively. Further, in F/M-vaccinatedJ ${alpha}$ 18^–/– mice, similar to WT mice, no IL-4-producingCD8⁺ T cells were detected by peptide Pb9 ELISPOT assays inthe liver or spleen above low naive background levels (datanot shown).

Prime-boost poxvirus vaccination activates ${alpha}$ -GalCer responsive V ${alpha}$ 14iNKT cells and NK cells in the liver. Since V ${alpha}$ 14iNKT cells promoted vaccine-induced CD8⁺ T cells inthe absence of ${alpha}$ GalCer, we tested whether attenuated poxvirusesthemselves exerted nonspecific influence on the hepatic andsplenic populations of V ${alpha}$ 14iNKT and NK cells after intradermalvaccination. To this end, we analyzed cell numbers and V ${alpha}$ 14iNKTcell cytokine production. The frequencies of hepatic CD1d/ ${alpha}$ -GalCertetramer⁺/TCRß⁺ V ${alpha}$ 14iNKT cells (percentage of all TCRß⁺cells) were reduced 14 and 20 to 25 days, but not 30 days, afterthe boost compared to naive mice (Fig. 2A and B). This reductionwas also observed after administration of the non-CSP-expressingvirus constructs (FP9lacZ/MVAlacZ) (Fig. 2A) and 14 days aftersingle immunizations (data not shown). Splenic V ${alpha}$ 14iNKT cellswere not affected (data not shown). CD1d/ ${alpha}$ -GalCer tetramer⁺/TCRß⁺V ${alpha}$ 14iNKT cells were CD8^– (Fig. 2B). DX5⁺/CD3^– NKcell frequencies were similarly reduced in the liver 14 and25 days postvaccination (Fig. 2C), but not in spleens (3 to5% of lymphocytes [data not shown]).

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FIG. 2. Systemic activation of V ${alpha}$ 14iNKT and NK cells in the livers of BALB/c mice by intradermal F/M vaccination. (A) Hepatic CD1d/ ${alpha}$ -GalCer tetramer⁺/TCRß⁺ V ${alpha}$ 14iNKT cell frequencies (gated as shown in panel B) by FACS analysis 14 days (D14) to 30 days after vaccination with the malaria vaccines or with empty control viruses (FP9lacZ/MVAlacZ). Pooled data from eight experiments, each including naive mice (n = 3 to 4/group) are presented. (B) Representative FACS dot plots of V ${alpha}$ 14iNKT cells on day 25 after F/M vaccination from panel A, with the percentages of positive cells displayed in quadrants. Gating first on lymphocytes (R1, upper dot plot) yielded CD1d/ ${alpha}$ -GalCer tetramer⁺/TCRß⁺ cells (V ${alpha}$ 14iNKT cells) in the upper right quadrant (middle dot plot). V ${alpha}$ 14iNKT cell frequencies in panel A are calculated as a percentage of these double tetramer⁺/TCRß⁺ cells from the sum of all TCRß⁺ cells (upper and lower right quadrant, middle dot plot). A second gating on all TCRß⁺ cells (R2, middle dot plot) demonstrates tetramer⁺ cells to be CD8^– (lower dot plot). (C) Hepatic NK cell frequencies before and after vaccination as in panel A, as determined by FACS analysis. (D and E) Hepatic ( ${blacksquare}$ ) and splenic () ex vivo IL-4 (D) and IFN- ${gamma}$ (E) V ${alpha}$ 14iNKT-cell responses to ${alpha}$ -GalCer, as measured by ELISPOT assay, from naive mice and mice 25 and 34 days after F/M vaccination (n = 4/group). The results from one representative experiment out of two performed are shown. Results are means ± the SEM; statistical analysis was done as described for Fig. 1.

Upon ex vivo stimulation with ${alpha}$ -GalCer in ELISPOT assays, wefound that hepatic V ${alpha}$ 14iNKT cells were activated to produce IL-4and IFN- ${gamma}$ within 25 days after F/M vaccination (Fig. 2D and E).The frequency of IL-4-producing liver V ${alpha}$ 14iNKT cells was increasedtwofold (Fig. 2D), and that of IFN- ${gamma}$ producers was increasedfivefold (Fig. 2E) in comparison to naive mice. Although therelative vaccine-induced activation of IFN- ${gamma}$ producers was morepronounced, IL-4-secreting liver V ${alpha}$ 14iNKT cells greatly outnumberedIFN- ${gamma}$ secretors in both naive and immunized mice at a ratio of75:1 and 30:1, respectively. In clear contrast to the liver,IL-4- and IFN- ${gamma}$ -producing ${alpha}$ -GalCer responsive V ${alpha}$ 14iNKT cells weremuch less frequent in the spleens of naive mice and not enhancedby vaccination. Splenic IL-4 producers were even reduced 25days postvaccination, but they also outnumbered IFN- ${gamma}$ secretorsin naive mice (90:1) and less so in immunized mice (20:1). At34 days postvaccination, the cytokine production of hepaticV ${alpha}$ 14iNKT cells had returned to naive levels (Fig. 2D and E).

V ${alpha}$ 14iNKT cells do not improve, but partially diminish, protection rates after sporozoite challenge. F/M-vaccinated WT and V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/–mice were challenged with P. berghei sporozoites in order toevaluate whether such differences in the magnitude of specificT-cell responses between the strains and the absence or presenceof poxvirus-activated V ${alpha}$ 14iNKT cells affected protection rates.Challenges were performed 10, 20, and 40 days after vaccinationto test the influence of short-lived vaccine-activated V ${alpha}$ 14iNKTcells at days 10 and 20 (Fig. 2A) or nonactivated V ${alpha}$ 14iNKT cells(day 30, Fig. 2A) on protection. After the first challenge atday 10, WT and J ${alpha}$ 18^–/– mice were similarly protectedat a rate of 80 to 90% with no difference in the time to parasitemiacompared to matched nonvaccinated controls (Fig. 3A). The protectionrates dropped rapidly in both vaccinated strains to below 45%when challenged 20 days postimmunization (Fig. 3B). The levelof protection was still significantly higher in vaccinated thanin nonvaccinated J ${alpha}$ 18^–/– mice but not in WT mice.Protection rates also declined to below 45% after rechallengeat day 40 in mice of both strains previously protected by vaccinationand were better in vaccinated J ${alpha}$ 18^–/– mice comparedto pooled nonvaccinated KO controls (Fig. 3C).

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FIG. 3. Protection rates after sporozoite challenge of vaccinated BALB/c WT ( ${blacksquare}$ ) and V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/– ( ${square}$ ) mice. (A) Challenge 10 days after F/M immunization or infection of nonimmunized control BALB/c WT (•) and J ${alpha}$ 18^–/– ( ${circ}$ ) mice by intravenous injection of 1,000 live sporozoites (n = 15 [ ${blacksquare}$ ], 17 [ ${square}$ ], 8 [•], or 6 [ ${circ}$ ]). CIs significant for comparison of immunized versus control mice were as follows: WT mice (39.2 to 92.5%) and J ${alpha}$ 18^–/– mice (30.8 to 90.4%). (B) Challenge 20 days after immunization. Data were pooled from two experiments (n = 6 [ ${blacksquare}$ ], 7 [ ${square}$ ], 6 [•], or 9 [ ${circ}$ ]). The CI values were significant only for immunized versus control J ${alpha}$ 18^–/– mice (2.5 to 75%). (C) Rechallenge of some of the mice, which were protected in panel A, at day 40 postimmunization (n = 10 [ ${blacksquare}$ ], 9 [ ${square}$ ], 4 [•], or 3 [ ${circ}$ ]); there was a significant difference between vaccinated animals and nine pooled KO controls (5.1 to 73.3%). Parasitemia was monitored by peripheral blood films; protected mice were negative on day 13.

Kinetics of vaccine-induced hepatic IFN- ${gamma}$ ⁺ CD8⁺ T cells correlate with TNF- ${alpha}$ ⁺ CD8⁺ T cells in response to sporozoite challenge and are influenced by V ${alpha}$ 14iNKT cells. Next, we tested whether hepatic IFN- ${gamma}$ - and TNF- ${alpha}$ -producing CD8⁺T cells responded to sporozoite challenge after vaccinationdependent on V ${alpha}$ 14iNKT cells. In both WT and V ${alpha}$ 14iNKT-cell-deficientJ ${alpha}$ 18^–/– mice the kinetics of IFN- ${gamma}$ -producing CD8⁺T cells were similar to those of TNF- ${alpha}$ producers in the early(day 1) and late (day 9) response to challenge, but were differentbetween the strains, and were therefore influenced by V ${alpha}$ 14iNKTcells (Fig. 4). In V ${alpha}$ 14iNKT cell-deficient mice, hepatic TNF- ${alpha}$ producers exceeded IFN- ${gamma}$ producers before (Fig. 1B and C) andafter challenge (Fig. 4C), peaked 1 day after challenge at around500 to 1,000 SFC/million, and declined to a level similar tothat of WT mice after 1 week (Fig. 4A and B). The kinetics weredifferent in WT mice because the levels of hepatic (Fig. 4A and B)and splenic (data not shown) IFN- ${gamma}$ -secreting (Fig. 4A)and TNF- ${alpha}$ -secreting (Fig. 4B) CD8⁺ T cells markedly declinedwithin 1 week; in some livers this occurred within 1 day afterchallenge. This reduction also implied a relative shift towardIFN- ${gamma}$ production (Fig. 4C). In the spleens, prechallenge differences(Fig. 1D) between WT and KO mice disappeared (Fig. 4D), butno significant reduction and therefore redistribution of theseCD8⁺ T cells to the liver occurred.

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FIG. 4. Different kinetics of hepatic IFN- ${gamma}$ - and TNF- ${alpha}$ -producing CD8⁺ T cells in vaccinated BALB/c WT ( ${blacksquare}$ ) and vaccinated V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/– () mice after sporozoite challenge. (A and B) Peptide Pb9-specific CD8⁺-T-cell responses were measured 20 days after F/M immunization before challenge (day 0 [D0]) and 1 and 9 days after challenge (n = 4) in IFN- ${gamma}$ (A) and TNF- ${alpha}$ (B) ELISPOT assays. (C and D) Comparison between these IFN- ${gamma}$ and TNF- ${alpha}$ responses in the liver (C) and spleen (D) 1 day after challenge. The results in panels A and B include some data from Fig. 2. Values are means ± the SEM; statistical analysis was done as in Fig. 1. The results for one representative experiment out of two performed are shown.

Hepatic pre-erythrocytic-stage antigen-specific IFN- ${gamma}$ and TNF- ${alpha}$ CD8⁺ T-cell responses are stronger in protected than parasitemic mice. Since the kinetics of both IFN- ${gamma}$ and TNF- ${alpha}$ -producers altered withchallenge, we further investigated how this related to protectionand patency. After challenge, lymphocytes infiltrated the liver(Fig. 5A), particularly strongly with patent infection in WTand V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/– mice (Fig. 5B).This influx was associated with increasing TNF- ${alpha}$ ⁺ and decreasingIFN- ${gamma}$ ⁺/CD8⁺-T-cell numbers in mice with delayed parasitemia (partialprotection) and was associated with the reverse in unprotectedmice (Fig. 5C). At 13 days postchallenge IFN- ${gamma}$ ⁺/CD8⁺ T cellspredominated irrespective of protection status (Fig. 5D). Vaccination-induceddouble-positive (IFN- ${gamma}$ ⁺/TNF- ${alpha}$ ⁺) CD8⁺ T cells were particularlyenhanced—in absolute number and frequency—in liversof fully protected rechallenged WT mice (Fig. 5D; 2,481 versus122), as well as J ${alpha}$ 18^–/– mice, compared to parasitemicmice (Fig. 5E; 2,298 versus 84) and compared to postvaccinationlevels (Fig. 1A and Fig. 5D; 2,481 versus 1,180 CD8⁺ T cells).These cells accounted for 30% of CD8⁺ T cells, whereas 60% producedIFN- ${gamma}$ and 10% produced TNF- ${alpha}$ alone (Fig. 5D). Such populationsof double-positive T cells were also observed in protected mice9 days after one challenge (data not shown). After 1 week ofparasitemia, the absolute number of single and double cytokine-producingCD8⁺ T cells was strongly reduced and, of those, only 7% expressedboth cytokines, 77% expressed IFN- ${gamma}$ alone, and 17% expressedTNF- ${alpha}$ alone (Fig. 5D). These data show that double-positive TNF- ${alpha}$ ⁺/IFN- ${gamma}$ ⁺CD8⁺ T cells in the liver were more strongly associated withprotection than single-positive IFN- ${gamma}$ ⁺ (OR = 6.56, P < 0.01)or TNF- ${alpha}$ ⁺ CD8⁺ T cells (OR = 6.11; P < 0.01). The same associationwas observed in J ${alpha}$ 18^–/– mice with lower frequenciesof double IFN- ${gamma}$ ⁺/TNF- ${alpha}$ ⁺ cells for total lymphocytes than CD3⁺/CD8⁺or CD3⁺/CD8^– T cells (Fig. 5E). The spleens of KO micecontained very few double-positive IFN- ${gamma}$ ⁺/TNF- ${alpha}$ ⁺ CD8⁺ T cellsafter challenge, and in WT spleens they were decreased frompostvaccination levels (Fig. 1E) independent of the protectionstatus (data not shown). Furthermore, the livers of protectedKO mice contained more single TNF- ${alpha}$ ⁺ and IFN- ${gamma}$ ⁺ CD8⁺ T cells thanthose of protected WT mice (Fig. 5D and E).

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FIG. 5. Protection is associated with stronger hepatic peptide Pb9-specific IFN- ${gamma}$ and TNF- ${alpha}$ CD8⁺-T-cell responses and weaker liver lymphocytosis than patent infection. (A) Absolute liver lymphocyte frequencies before (day 0 [D0]) and at days 1 and 9 days postchallenge of BALB/c WT and J ${alpha}$ 18^–/– mice (n = 4); challenge was performed 20 days after F/M vaccination. (B) Samples from panel A (day 9), separated into protected (p., n = 2) and unprotected (n.-p., n = 2) mice, including a delay in time to parasitemia as partial protection. (C) Examples of absolute peptide Pb9-specific liver ELISPOT responses at day 9 in WT mice from panel B, including a 2-day delay until day 8, with a read-out on the second parasitemic day, day 9. Means ± the SEM are shown; statistical analysis was done as in Fig. 1. (D and E) Pb9-stimulated pooled hepatic MNC from protected (n = 4, upper row) and unprotected (n = 4, bottom row) WT (D) and J ${alpha}$ 18^–/– (E) mice 13 days after rechallenge (rechallenge was performed at day 40 postvaccination). Absolute positive cells per million lymphocytes in the respective quadrants, calculated with percentages of gated CD8⁺/CD3⁺ and CD8^–/CD3⁺ subpopulations, are demonstrated below the FACS analysis profiles.

Furthermore, nonspecific hepatic background production of IFN- ${gamma}$ and TNF- ${alpha}$ was detected in ELISPOT assays and ICS in all infected,but particularly in protected mice, more in KO than in WT mice,when the total absolute frequencies were compared. Most of itderived from CD3^– lymphocytes and some CD8^– T cells(Fig. 5D and E).

ICS isotype controls of hepatic MNC from protected mice showedvery low or no nonspecific staining of the cytokines (rat IgG1),CD8 (rat IgG2a) (Fig. 1F), or CD3 (hamster IgG1) (data not shown).

Sporozoite challenge affects hepatic V ${alpha}$ 14iNKT cells and NK cells. Since non-T-cell-related cytokine expression was pronouncedin protected mice, we examined whether challenge influencedV ${alpha}$ 14iNKT cells or NK cells. Significantly more hepatic V ${alpha}$ 14iNKTcells secreted IFN- ${gamma}$ 6 days after challenge compared to 1 dayafter challenge and compared to mice that were vaccinated butnot challenged (Fig. 6A) or to naive WT mice (Fig. 2E). At thesame time, hepatic IL-4-producing V ${alpha}$ 14iNKT cells decreased froma ratio of 30:1 (300,000:10,000) at 1 day postchallenge to 10:1(200,000: 20,000) at 6 days (Fig. 6B). The total numbers ofhepatic CD1d tetramer/ ${alpha}$ -GalCer⁺ or IL-4/IFN- ${gamma}$ -expressing splenicV ${alpha}$ 14iNKT cells were not affected (data not shown). Concomitantly,DX5⁺/CD3^– NK cells increased twofold in livers and converselydeclined in spleens 6 days after challenge in vaccinated WTand V ${alpha}$ 14iNKT-cell-deficient J ${alpha}$ 18^–/– mice, findingsequal to those observed in naive infected mice. More NK cellsappeared in the livers of naive and vaccinated J ${alpha}$ 18^–/–mice than in those of WT mice at the first day postchallenge(P = 0.023 and 0.001, respectively). In contrast to WT mice(Fig. 2C and 6C), immunization did not reduce the numbers ofhepatic NK cells in V ${alpha}$ 14iNKT-cell-deficient mice (Fig. 6D).

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FIG. 6. Sporozoite challenge shifts the cytokine production of V ${alpha}$ 14iNKT cells and influences NK cells in the liver. (A and B) IFN- ${gamma}$ (A) and IL-4 (B) V ${alpha}$ 14iNKT cell responses to ${alpha}$ -GalCer, measured by ELISPOT assay, in the livers ( ${blacksquare}$ ) and spleens () of BALB/c WT mice, F/M vaccinated on day 25 (D25) and examined on days 1 and 6 after challenge (n = 4). This is the same experiment as in Fig. 1. (C and D) NK cell frequencies, as determined by FACS analysis, in the livers and spleens of WT (C) and J ${alpha}$ 18^–/– (D) mice. Mice were challenged 25 or 30 days after vaccination, or nonvaccinated mice were examined before infection (day 0, n = 8) or 1, 6, or 8 days postinfection (n = 4). Means ± the SEM are shown; statistical analysis was performed as in Fig. 1. Results from a representative experiment out of two performed are shown.

In summary, infection induced a Th1-directed shift of cytokine-producingV ${alpha}$ 14iNKT cells. Immunization and challenge affected NK cellsdifferently in the absence or presence of V ${alpha}$ 14iNKT cells.

DISCUSSION

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Discussion

Recently, glycolipid-activated V ${alpha}$ 14iNKT cells have been reportedto play an adjuvant-like role in enhancing certain types ofvaccination against liver-stage malaria (19), but it is unclearwhether recombinant vaccines alone affect V ${alpha}$ 14iNKT cells. Thereare very few kinetic studies of innate, non-macrophage-relatedresponses after vaccination. For example, the killed influenzavaccine and combined mumps-measles-rubella vaccine enhance NKcell activity for 2 to 30 days (38, 41). The present study demonstratesthat intradermal prime-boost vaccination with the attenuated,nonreplicating recombinant poxviruses FP9/MVAPbCSP systemicallyactivates the already prevailing IL-4, as well as IFN- ${gamma}$ productionof hepatic, but not splenic, V ${alpha}$ 14iNKT cells in BALB/c mice andinduces a temporary reduction in frequencies of V ${alpha}$ 14iNKT andNK cells. The main mechanism for this reduction may be activation-inducedcell death because hepatic V ${alpha}$ 14iNKT cells, and in turn transactivatedNK cells, are particularly prone to this, e.g., after in vivostimulation with ${alpha}$ -GalCer (37). In comparison, we found a longerand ${alpha}$ -GalCer-independent activation of both populations ex vivoin response to ${alpha}$ GalCer for approximately 25 days after immunization.This activation by ${alpha}$ GalCer in ELISPOT assays (19) is unlikelyto involve bystander activation of CD8⁺ or CD4⁺ T cells because ${alpha}$ GalCer cannot indirectly stimulate more hepatic CD8⁺ T cellsthan peptide Pb9 itself (ca. 10,000 versus 1,000 SFC), a possibilityalso countered by the low numbers in CD8⁺/CD4⁺ T-cell- and NK-cell-richspleens. Bystander activation was also not observed in a similarmalaria vaccination model with nonseparated peptide-stimulatedcells (9). Further, we detected no peptide Pb9-specific vaccine-inducedIL-4-producing CD8⁺ T cells in the liver or spleen. Interestingly,IL-4-producing T cells predominate in human blood 14 days aftersubcutaneous measles virus vaccination (47), and repeated invivo administrations of ${alpha}$ -GalCer polarize splenic V ${alpha}$ 14iNKT cellstoward IL-4 (6). Here, two consecutive poxvirus vaccinationsinduced a proportional, but not a complete, Th1 shift in theliver because IL-4-producing V ${alpha}$ 14iNKT cells prevailed. This supportsthe concept of the liver as a Th2-driving environment (10, 27)and might be relevant for vaccine design and studies with multiplepoxvirus booster immunizations at short intervals, which haveoccasionally revealed reduced vaccine efficacy (3).

We assessed whether such activated V ${alpha}$ 14iNKT cells and their absencein J ${alpha}$ 18^–/– mice could influence vaccine immunogenicityand protection. Nonactivated V ${alpha}$ 14iNKT cells have no effect onsporozoite-induced memory responses, while ${alpha}$ -GalCer-activatedV ${alpha}$ 14iNKT cells enhance protection mediated by IFN- ${gamma}$ CD8⁺ T-cellmemory responses to recombinant Sindbis virus, adenovirus, andirradiated sporozoite malaria liver-stage vaccines (19). Ourfindings extend these data by demonstrating that not only IFN- ${gamma}$ -secretingbut also TNF- ${alpha}$ -secreting CSP (peptide Pb9)-specific CD8⁺ T cellswere increased in the spleen and more so in the liver in a synergisticmanner by V ${alpha}$ 14iNKT cells independently of ${alpha}$ -GalCer, because bothwere reduced in poxvirus-vaccinated J ${alpha}$ 18^–/– micecompared to WT mice. Sufficient backcrossing of the KO miceexcludes the possibility that CD8⁺-T-cell numbers were influencedby differences in the genetic backgrounds of the lines (14).We propose that vaccine-activated IFN- ${gamma}$ - and IL-4-producing V ${alpha}$ 14iNKTcells are responsible for this intrinsic adjuvant effect ofpoxvirus vaccines. IFN- ${gamma}$ and IL-4 can promote the generationof antigen-specific Th1 cells (8, 17, 22). Interestingly, levelsof IL-4-secreting peripheral blood CD4⁺ T cells increase aftereach vaccination with attenuated sporozoites in volunteers,who show sustained protection (28).

As for protection, the overall protection rates after vaccination(vaccine efficacy) were lower here than in previous studies(45) using the intradermal route, which is currently used inmost clinical trials. The intradermal route, as well as improvedsporozoite isolation and infectivity, may contribute to this.However, the main efficacy results were that V ${alpha}$ 14iNKT-cell-deficientand WT mice were similarly well protected to 90% at the earliesttime point after vaccination, but at the later time points protectionwaned in >50% of mice of both strains, but vaccinated KOappeared to be better protected than vaccinated WT mice. Thisindicates, first, that nonspecific protective effects mediatedby virus-activated V ${alpha}$ 14iNKT cells can be ruled out. Parallelstudies by our laboratory show that empty control viruses donot protect mice (3, 45), which also excludes such effects.Second, the intrinsic adjuvant effect of attenuated poxvirusesmediated by V ${alpha}$ 14iNKT cells is not strong enough to improve protectionin WT mice despite an enlarged memory T-cell pool 3 weeks aftervaccination, in contrast to ${alpha}$ -GalCer-adjuvanted immunization(19). This supports other previous studies showing a dispensablephysiological role of V ${alpha}$ 14iNKT cells in protection against liver-stagemalaria (18, 39, 43). The slightly better protection of KO micemight be due to the absence of IL-4-producing V ${alpha}$ 14iNKT cells,promoting a Th1-polarized liver environment, indicated by highernumbers of NK cells as well as of CD8⁺ T and CD3^– cellsexpressing IFN- ${gamma}$ or TNF- ${alpha}$ intracellularly. In line with this,a shift toward protective IFN- ${gamma}$ responses in the liver occursin naive infected IL-4 KO or IL-4 receptor KO BALB/c mice (40).

These results support the current view that IFN- ${gamma}$ -secreting CD8⁺(and CD4⁺) T cells are the best-defined correlate of protectionagainst liver-stage malaria. Furthermore, this is the firstreport of the induction of pre-erythrocytic-stage antigen-specificTNF- ${alpha}$ -producing CD8⁺ T cells in the liver by vaccination, detectedby ELISPOT assay and ICS in both liver and spleen. This inductionis specific because vaccination with the empty control virusesdoes not yield peptide Pb9-specific cytokine producers (3),as also supported by the negative test controls. One previousstudy reports intracellularly stained TNF- ${alpha}$ in splenic CD8⁺ memoryT cells induced by malaria DNA recombinant vaccinia virus vaccines(46). TNF- ${alpha}$ -producing antigen-specific CD8⁺ T cells have mainlybeen described for bacterial and viral infections (21, 48).Here, TNF- ${alpha}$ -producing CD8⁺ T cells correlated with IFN- ${gamma}$ secretorsafter vaccination and in the early and late response to sporozoitechallenge. Further, CD9⁺ T cells that produce both IFN- ${gamma}$ andTNF- ${alpha}$ were associated with vaccine-induced protection, sincethey accumulated in greater numbers in livers of protected WTand V ${alpha}$ 14iNKT-cell-deficient mice compared to unprotected miceand to postvaccination levels. Blood-stage parasites, accumulatingin the livers of parasitemic mice, could conceivably accountfor the reduction in unprotected mice, due to some cross-reactivitywith CSP (1) and the death of activated liver lymphocytes (10),but not for the shifts observed 1 day after challenge and inprotected versus vaccinated mice. Therefore, we suggest thatdouble-expressing, as well as single-expressing, T-cell populationsshould be further investigated as possible correlates of protectionfor liver-stage malaria. However, further studies are neededto prove their protective role. Interestingly, such IFN- ${gamma}$ ⁺/TNF- ${alpha}$ ⁺liver-stage-specific T cells were recently found to be enhancedin the blood of protected, vaccinated volunteers (S. Kortenet al., unpublished data).

Local intrahepatic memory CD8⁺ T cells are thought to be mostrelevant for protection against liver-stage malaria (4). Theprotective threshold levels for antigen-specific hepatic CD8⁺T cells that we present here are novel and might be helpfulfor further vaccine studies. For BALB/c WT spleens, the estimatedlevel for protection is ca. 500 IFN- ${gamma}$ -secreting SFC/million splenocytes,which are specific for one peptide (44). Our data suggest aprotective hepatic threshold level of 500 SFC/million lymphocytesspecific for peptide Pb9 because this level was also achievedhere in livers of KO mice for both cytokines together afterimmunization and for each cytokine 1 day after challenge ofimmunized KO mice. Infectious sporozoites induce a peak reactivityof hepatic effector memory CD8⁺ T cells within 1 to 6 h, whereashepatic central memory CD8⁺ T cells are conscripted into effectorswith some delay (4). This might apply to the different postchallengekinetics of hepatic CD8⁺ T cells in WT and V ${alpha}$ 14iNKT-cell-deficientmice. The livers of WT mice might have contained a greater effectorCD8⁺-T-cell pool, that quickly responds and contracts 1 dayafter challenge, whereas in KO mice central memory CD8⁺ T cellshad to be conscripted into effectors and therefore peaked 1day after challenge. Splenic memory T cells were not significantlyredistributed to the liver early after challenge, suggestingthat hepatic memory T cells were the main effectors. Later redistributionsfrom the spleen would have no protective effect, since CSP isnot newly expressed by hepatic stages (5). Second, in the presenceof V ${alpha}$ 14iNKT cells, which rapidly activate NK cells (7), the cytokinecascade might be more potent and activate protective effectorCD8⁺ T cells faster.

In conclusion, maximizing local hepatic or splenic memory CD8⁺-T-cellpools specific for one antigen alone does not automaticallyimprove protection. Higher levels of IFN- ${gamma}$ producers can protectbetter, but this was shown for total, not single peptide specific,effector memory IFN- ${gamma}$ -producing CD8⁺-T-cell pools after vaccinationwith gamma-irradiated sporozoites (4). Therefore, our findingsmay prove generally valuable for evaluating vaccine efficacyand designing more effective vaccines against pre-erythrocytic-stagemalaria.

ACKNOWLEDGMENTS

This study was sponsored by the Wellcome Trust. S.K. was fundedby the German Research Foundation (DFG). A.V.S.H. is a WellcomeTrust Principal Research Fellow.

We thank Vincenzo Cerundolo for assistance with the CD1d/ ${alpha}$ -GalCertetramer, Kirin Brewery for providing ${alpha}$ GalCer, Jacqui Mendozaand Volker Heussler for supplying P. berghei-infected mosquitoes,Britta Urban for technical assistance, and Michael Walther forstatistical advice.

FOOTNOTES

* Corresponding author. Mailing address: Department of Immunology, Bernhard-Nocht-Institute for Tropical Medicine, Bernhard-Nocht-Str. 74, 20359 Hamburg, Germany. Phone: 49-40-42818-412. Fax: 49-40-42818-400. E-mail: korten{at}bni-hamburg.de.

Editor: S. H. E. Kaufmann

REFERENCES

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