- Open Access
Immunization with different Pf AMA1 alleles in sequence induces clonal imprint humoral responses that are similar to responses induced by the same alleles as a vaccine cocktail in rabbits
© Kusi et al; licensee BioMed Central Ltd. 2011
Received: 23 December 2010
Accepted: 14 February 2011
Published: 14 February 2011
Antibodies to key Plasmodium falciparum surface antigens have been shown to be important effectors that mediate clinical immunity to malaria. The cross-strain fraction of anti-malarial antibodies may however be required to achieve
strain-transcending immunity. Such antibody responses against Plasmodium falciparum apical membrane antigen 1 (Pf AMA1), a vaccine target molecule that is expressed in both liver and blood stages of the parasite, can be elicited through immunization with a mixture of allelic variants of the parasite molecule. Cross-strain antibodies are most likely elicited against epitopes that are shared by the allelic antigens in the vaccine cocktail.
A standard competition ELISA was used to address whether the antibody response can be further focused on shared epitopes by exclusively boosting these common determinants through immunization of rabbits with different Pf AMA1 alleles in sequence. The in vitro parasite growth inhibition assay was used to further evaluate the functional effects of the broadened antibody response that is characteristic of multi-allele vaccine strategies.
A mixed antigen immunization protocol elicited humoral responses that were functionally similar to those elicited by a sequential immunization protocol (p > 0.05). Sequential exposure to the different Pf AMA1 allelic variants induced immunological recall of responses to previous alleles and yielded functional cross-strain antibodies that would be capable of optimal growth inhibition of variant parasites at high enough concentrations.
These findings may have implications for the current understanding of the natural acquisition of clinical immunity to malaria as well as for rational vaccine design.
Malaria caused by parasites of the Plasmodium spp. continues to be a major public health problem with half of the world's population at risk of infection . The greatest risk of disease and fatality in Plasmodium falciparum-endemic areas occurs in children under 5 years and in first-time pregnant women. Natural immunity to clinical malaria is believed to develop in an age- and exposure-dependent manner, after repeated infection by a number of (different) parasite strains [2–4]. Even in adults who have had several parasite encounters, acquired clinical immunity is partial and is believed to be dependent on constant or periodic exposure to low-level parasitaemia [3, 5].
The natural ability to acquire immunity to malaria, although partial, is a strong indication of the feasibility of developing at least an anti-disease vaccine directed against the blood stages of Plasmodium. Antigenic variation in immunogenic parasite targets however provides an immune escape route for parasites. Polymorphism in such well-known vaccine targets as the Merozoite Surface Proteins (MSPs) and Apical Membrane Antigen 1 (AMA1) have been associated with host immune pressure on parasites [6–10]. This presents malaria vaccine researchers with a formidable challenge since immunization with one variant of these polymorphic antigens induces antibodies that show limited cross-inhibition/recognition of parasites expressing other allelic variants of the same antigen. This has been demonstrated extensively in animal models [11, 12] and to some extent in human field studies [13–16].
There is growing interest in multi-allele/multi-antigen malaria vaccines and the potential of such vaccines for the induction of broad inhibitory antibody responses has been demonstrated [17–19]. The broadened response most likely results from diluting out strain-specific epitopes in the antigen mixture, with the bulk of remaining epitopes being those that are common to the vaccine component alleles .
The hypothesis that immunization of rabbits with different Pf AMA1 alleles in sequence would result in boosting of only antibodies to epitopes that are common to all antigens was tested in this study. Antibodies to highly specific epitopes would not be boosted, and this is expected to further increase the proportion of induced cross-strain antibodies in comparison with antibodies induced by a multi-allele vaccine that incorporates the same allelic antigens. Such a mechanism of cross-strain antibody production would be based on the concept of original antigenic sin (clonal imprinting). Original antigenic sin results when prior exposure to one strain/antigen diverts the antibody response to shared epitopes following exposure to a second closely related strain/antigen such that the newly elicited antibodies still react strongly with the priming antigen [21–23]. A sequential immunization protocol may mimic the development of natural clinical immunity and provide some insight into its acquisition in the field where over time an individual is exposed (sequentially) to a number of variant parasite strains. The generated data shows that a sequential immunization protocol may not be materially different from a mixed antigen protocol with respect to the proportions of elicited strain-specific and cross-strain antibodies. As expected, antibody production in the sequential immunization groups was through associative immune recall of previous antigen encounter. This data is relevant to the current understanding of the acquisition of clinical immunity against malaria in endemic areas, as well as for rational vaccine design.
Antigen production, rabbit immunization and antibody purification
The full ectodomain of the AMA1 allelic forms from P. falciparum strains FVO, HB3, 3D7 and CAMP, as well as the in silico-designed Di versity Co vering antigens (DiCo 1, DiCo 2 and DiCo 3) , were expressed as recombinant proteins in Pichia pastoris. The three DiCo proteins were all expressed with the FVO AMA1 prodomain, and all antigens were mutagenized at up to six potential N-glycosylation sites within the Pf AMA1 ectodomain. The expression, purification and characterisation of all antigens were as described previously .
Schedule indicating the order of Pf AMA1 antigen administration to rabbits.
Antigens and immunization
*Number of rabbits
4 (NA mix)
5 (DiCo mix)
Antibodies from final bleed sera were purified on Protein G Sepharose (GE Healthcare, Etten-Leur, The Netherlands) columns. Binding and elution buffers (Pierce, Rockford, IL) were used according to manufacturer's protocols. After elution, antibody eluates were filtered (0.22 μm), concentrated and exchanged into RPMI 1640 using pre-sterilized Amicon Ultra-15 tubes (30-kDa cutoff; Millipore, Ireland). The concentration of each antibody fraction was subsequently determined by a Nanodrop ND1000 spectrophotometer (Nanodrop Technologies, Wilmington, DE) using the IgG extinction coefficient, adjusted to 12 mg/ml and stored at -20°C until use.
ELISA and growth inhibition assays
Sera from all rabbits were titrated in a standardized ELISA on plates coated with recombinant AMA1 allelic antigens from FVO, HB3 or 3D7 parasite strains. Sera were also analysed with a harmonized competition ELISA protocol that has been described elsewhere . FVO, HB3 and 3D7 AMA1 proteins were used as capture antigens and FVO, HB3, 3D7 and CAMP AMA1 antigens were used as competitor antigens in all assays.
Protein G-purified IgG fractions from final bleed sera were tested for in vitro activity in parasite growth inhibition assays (GIAs). All IgGs were tested in triplicate on FCR3 (one amino acid difference in the pro-domain from the FVO strain, with ama1 GenBank accession no. M34553), NF54 (parent strain of the 3D7 clone with ama1 GenBank accession no. U65407), HB3 (accession no. U33277), 7G8 (accession no. M34555) and CAMP (accession no. M34552) parasite strains at a 2-fold serial dilution from 6 mg/ml in 96-well half area cell culture plates (Greiner, Alphen a/d Rijn, The Netherlands). Parasites were cultured under standard conditions (an atmosphere of 5% CO2, 5% O2, and 90% N2, 37°C), and all parasite strains were verified by PCR and restriction fragment length analysis of the Pf AMA1 antigen they express. Parasite cultures were mycoplasma-free and synchronized with 0.3 M Alanine, 10 mM Hepes, pH 7.5 before use in assays. Late trophozoite/early schizont stages at a parasitaemia of 0.3 ± 0.1% and 2% final haematocrit were used in all assays. The final culture volume was 50 μl/well and parasites were incubated for 42-46 h. Parasite growth was assessed by measuring parasite lactate dehydrogenase levels and plates were read at 655 nm after 30 min of development. Parasite growth inhibition was expressed as 100 - ((A 655 Sample - A 655 RBC)/(A 655 SZ - A 655 RBC)) × 100, where A 655 Sample is the OD655 for any test sample well, A 655 SZ is the average OD655 of schizont control wells included on each plate and A 655 RBC is the average OD655 of RBC control wells. The data is presented as the arithmetic mean% inhibition from each sample triplicate.
All analyses and graphics were made using the R statistical package (R Development Core Team, 2009, version 2.10.1). ELISA antibody titres in day 70 sera were log-transformed and compared between groups by one-way analysis of variance (ANOVA) followed by the pair-wise Tukey Honest Significant Difference post hoc test which applies a correction for multiple comparisons. Titres are also presented as dotplots superposed with boxplots indicating the median, lower and upper quartiles. Residual antibody binding (Y min ) for each competitor antigen in competition ELISA was estimated by a 4-parameter logistic fit with least squares approximation. The mean % depletion (100-Y min ) and corresponding 95% confidence intervals (95% CI) for each competitor antigen are presented for all immunization groups. GIA data is presented as the mean % growth inhibition ± standard error of mean per immunization group against the five parasite strains. Associations between antibody titre and the corresponding in vitro parasite growth inhibition levels were estimated with a four-parameter logistic fit. Differences were considered statistically significant at p < 0.05, or when the 95% CI of groups being compared did not overlap.
One of the 6 rabbits in the first immunization group (f3h) experienced pneumonia during the study and data from this rabbit was excluded from all analyses. Rabbits (n = 4) in one of the sequential groups (h3f, Table 1) were immunized in a different experiment.
Specificity of antibodies elicited with mixed allele and sequential allele immunization protocols
Mean % antibody depletion from FVO, HB3 and 3D7 AMA1-coated plates.
Gp 1 (f3h) n = 5
Gp 2 (hf3) n = 6
Gp 3 (h3f) n = 4
Gp 4 (NA mix) n = 6
Gp5 (DiCo mix) n = 6
98.5 (97.3 - 99.7)
95.9 (95.1 - 96.8)
98.2 (96.3 - 100.1)
96.8 (95.4 - 98.2)
97.6 (96.4 - 98.7)
93.2 (88.1 - 98.3)
90.4 (87.0 - 93.8)
93.2 (86.0 - 100.4)
90.6 (87.4 - 93.9)
91.3 (89.7 - 92.9)
84.5 (77.5 - 91.5)
75.5 (74.3 - 76.7)
76.6 (65.4 - 87.8)
70.4 (64.7 - 76.0)
77.0 (69.4 - 84.7)
78.7 (73.6 - 83.7)
70.3 (65.9 - 74.6)
74.2 (64.4 - 84.1)
70.3 (64.7 - 74.0)
84.0 (82.3 - 85.8)
87.5 (79.0 - 96.0)
86.0 (81.2 - 90.9)
91.4 (89.3 - 93.6)
86.6 (83.3 - 89.9)
84.1 (80.6 - 87.5)
96.1 (93.6 - 98.5)
97.5 (95.4 - 99.6)
98.2 (98.1 - 98.4)
96.7 (95.0 - 98.4)
95.6 (93.7 - 97.4)
86.7 (82.3 - 91.0)
84.3 (75.9 - 92.8)
77.9 (70.5 - 85.4)
73.7 (66.7 - 80.6)
74.7 (70.5 - 78.9)
76.8 (73.4 - 80.1)
68.5 (62.7 - 74.3)
74.4 (70.2 - 78.6)
66.8 (60.2 - 73.3)
81.2 (78.2 - 84.2)
83.0 (75.3 - 90.8)
91.8 (86.7 - 97.0)
91.3 (84.8 - 97.9)
73.2 (66.1 - 80.3)
86.9 (84.4 - 89.4)
89.3 (85.2 - 93.4)
95.9 (92.7 - 99.1)
94.1 (89.2 - 99.0)
83.6 (76.1 - 91.1)
88.7 (86.2 - 91.2)
100.2 (96.8 - 103.7)
98.2 (95.9 - 100.2)
96.8 (94.6 - 99.0)
95.8 (94.3 - 97.4)
97.1 (95.2 - 99.0)
79.5 (71.6 - 87.5)
82.0 (77.0 - 87.1)
85.7 (77.0 - 94.5)
71.0 (66.5 - 75.5)
89.2 (86.0 - 92.4)
Comparison of the three sequential immunization groups (f3h, hf3 and h3f) showed that though there were small differences (based on overlaps in 95% CI, Table 2) in the extent of heterologous antibody depletion, no clear trends emerged with respect to the order of antigen administration and the capture antigen used in assays. The three sequential immunization groups also showed detectable quantities of antibodies that were specific to each of the three vaccine Pf AMA1 alleles in all polyclonal pools on day 70, despite the fact that each allelic antigen was administered at only one of the three time points.
Comparisons across all groups showed that antibody depletion by heterologous competitor antigens was generally lowest in the NA mix immunization group compared to the three sequential immunization groups (f3h, hf3 and h3f, Table 2). The observed differences were however not always statistically significant since 95% CI sometimes overlapped. Antibody depletion by CAMP AMA1, an allele that was not in any of the vaccine formulations, was greatest for antibodies from the DiCo mix vaccine group compared to the other four groups in all assays (Table 2). CAMP AMA1 depletion of anti-DiCo mix antibodies was statistically significantly higher than that of anti-NA mix antibodies irrespective of the capture antigen, while differences between anti-DiCo mix antibodies and the sequential immunization groups were not always statistically significant (Table 2).
Functional capacity of antibodies elicited with mixed allele and sequential allele immunization protocols
Antibodies from the sequential (f3h, hf3 and h3f) and NA mix immunization groups generally showed a reduction in the extent of in vitro inhibition of "heterologous" parasite strains (CAMP, 7G8) compared to that of "homologous" strains (NF54, FCR3, HB3). Mean inhibition with antibodies from both the f3h (Gp 1) and NA mix (Gp 4) immunizations at 6 mg/ml were all higher against "homologous" strains (NF54, HB3, FCR3) compared to those against the CAMP and 7G8 strains (p < 0.0001, one-way ANOVA). Mean inhibition of antibodies from the hf3 group (Gp 2) were however only higher against HB3 strains when compared pair-wise with the "heterologous" strains (p = 0.006 for 7G8 and p = 0.005 for CAMP parasites, Tukey HSD). Antibodies from the h3f group (Gp 3) also showed higher mean inhibition against HB3 in comparison with the CAMP strain (p = 0.024, Tukey HSD). In contrast, antibodies from the DiCo mix group (Gp 5) showed a generally consistent level of inhibition of all five parasite strains (Figure 3). Mean growth inhibitions ranged from 47.2% against the CAMP strain to 66.9% against the HB3 strain at 6 mg/ml total IgG, and these were not statistically significantly different (p = 0.55, one-way ANOVA).
An effective malaria vaccine is expected to confer similar or better immunity to malaria-susceptible individuals compared to that of adults who are resident in endemic areas, but over a shorter period of time. In semi-immune adults, this level of anti-disease immunity is acquired after repeated infection with diverse parasite strains [2, 3]. Antibodies are key components of anti-disease immunity [26, 27], and the cross-strain fraction of anti-malarial antibodies may be important effectors against parasite strains that express diverse polymorphic antigens [7, 14, 28]. The main objectives of this study were to compare sequential and mixed Pf AMA1 immunization protocols for the proportions of functional cross-strain antibodies they induce in rabbits, and to further demonstrate the specificity broadening effects of such vaccination strategies.
Statistically similar levels of antibodies were induced with all vaccine formulations, irrespective of the order of antigen administration (Figure 1). This suggests that the order of antigen exposure may not influence the levels of elicited antibodies. For sequential immunization groups, this shows that "booster" responses were associative recall responses of previous allele vaccinations, and antibodies were mostly to epitopes that are shared by vaccine alleles. This is consistent with published data on both cellular and humoral immune responses to other polymorphic malaria antigens [7, 29–31], and is a well-established phenomenon in immune responses to other parasitic and viral infections [21, 22, 32–34].
Antibody depletion data from competition assays showed marginally higher proportions of cross-strain antibodies in some sequential immunization groups compared to the NA mix group (Table 2). Since significance was achieved only in some instances and there were no observable trends with respect to capture and competitor antigens, the order of antigen administration may only marginally influence the ultimate specificity of antibodies on day 70. The three-antigen DiCo mix vaccine generally yielded higher proportions of cross-strain antibodies compared to the three-antigen NA mix vaccine, especially against the out-group competitor antigen CAMP (Table 2). This suggests that the three DiCo antigens together present a greater proportion of epitopes that induce broad-reacting antibodies, and affirms the specificity broadening properties of the DiCo vaccine approach [9, 35].
The determination of strain-specific antibodies against vaccine alleles in sequential immunization groups on day 70 (Table 2) suggests that immunization with a single allele does induce long-lived responses. This may reflect the persistence of strain-specific antibodies that were induced after antigen administration on day 0 (first antigen), 28 (second antigen) or 56 (third antigen). Alternatively, memory B cells to these specific antibody epitopes in previous vaccine alleles could be activated by the altered, corresponding low affinity epitopes on subsequently administered Pf AMA1 alleles, leading to high affinity secondary responses against the cognate epitopes. The latter phenomenon is in agreement with the mechanism underlying original antigenic sin, and supports the existence of a continuum of antibody specificities . It must be noted that the specificity of an antibody for an antigen is directly related to the affinity of the antigen-antibody interaction hence an antibody that is "specific" to one Pf AMA1 allele may indeed have very low affinity for other alleles.
Data from in vitro growth inhibition assays was consistent with the observations in ELISA. The similar inhibition of FCR3, HB3 and NF54 parasite strains by purified antibodies from sequential immunization (f3h, hf3 and h3f) and NA mix groups suggests that comparable levels of functional antibodies against all three parasite strains were present on day 70, irrespective of the order of antigen administration (Figure 3). This confirms the induction of antibodies mostly to shared epitopes based on the original antigenic sin phenomenon [7, 22].
The observed higher inhibition of parasite strains expressing the vaccine alleles compared to the out-group strains (CAMP, 7G8) may be attributed to the generally low levels of antibodies induced in all immunization groups. A similar observation was made in an earlier study where low titres of antibodies elicited against DiCo mix in Montanide IMS resulted in lower in vitro parasite inhibition levels compared with the higher antibody levels against DiCo mix in two other adjuvants . ELISA antibody titres and parasite inhibition levels in the present study are intermediate between those of anti-DiCo mix antibodies elicited in the previous study with Montanide IMS on the one hand and CoVaccine HT™/Montanide ISA 51 on the other hand. Similar proportions of cross-strain antibodies were measured in both studies despite the different absolute antibody titres. At such low antibody titres, high avidity strain-specific antibodies, which form a small proportion of elicited antibodies, most likely augment the functional effects of cross-strain antibodies against the respective homologous parasite strains. This fraction of strain-specific antibodies would however have very low avidities for AMA1 of the CAMP and 7G8 strains, resulting in lower levels of inhibition of these strains (Figure 3). Thus high titres of functional cross-strain antibodies are required to optimally inhibit "heterologous" strains. At high antibody titres, the additional inhibitory activity of any strain-specific antibodies against "homologous" parasites would put the overall inhibitory effect in the upper plateau region of the antibody binding-function curve (Figure 4). A possible limitation here however, is that some parasites, here the HB3 strain, may be inherently easier to inhibit than others, and this could mask the effect of vaccine responses described. Similar effect has been described for D10 parasites, which can be inhibited better with anti-3D7 AMA1 antibodies compared to inhibition of the homologous 3D7 strain [36, 37].
Although anti-DiCo mix antibodies least inhibited the three "homologous" strains, these antibodies performed as well against the two out-group parasite strains as antibodies from all other vaccine formulations. Additionally, unlike the other vaccine formulations, anti-DiCo mix antibodies showed consistent inhibition of all parasite strains. This consistency, coupled with the significantly higher depletion of anti-DiCo antibodies by the out-group CAMP AMA1 competitor antigen when compared to anti-NA mix antibodies, suggests that DiCo mix may have a slight advantage as a vaccine candidate, since AMA1 from culture-adapted strains may not necessarily be encountered in the field.
The current in vitro growth inhibition data may seem inconsistent with our earlier published data , where rabbit antibodies elicited with a three-antigen (FVO, HB3, 3D7 AMA1) vaccine in Montanide ISA720 inhibited a heterologous parasite strain (CAMP) to a similar extent as the three "homologous" strains. This can however be explained by the fact that data from the earlier study was based on a single sample per immunization group, with antibody titres that were 2-4 times higher than the average antibody titres in the study under discussion. The greater potency of the adjuvant used in the earlier study may partially account for the higher titres. Additionally, the earlier study used an immunization protocol (4 vaccine doses on days 0, 28, 56 and 82, exsanguination on day 95) that is different from the one used in the current study (3 doses on days 0, 28 and 56, exsanguination on day 70). The extra booster dose, as well as the longer study period, could account partially for the higher functional antibody titres, which were most likely at saturation levels. It must be noted that single allele immunizations with FVO, HB3 and 3D7 AMA1 alleles in the previous study also resulted in similar antibody titres to that of the three-antigen mixed allele vaccine but failed to achieve the same level of in vitro inhibition of heterologous parasites as the mixed allele vaccine . Moreover, mixed allele vaccine antibodies from both studies showed similar binding specificities for the component antigens. Thus high titres of cross-strain antibodies are necessary for significant inhibition of variant parasites, and this is consistent with earlier published literature in both in vitro and in vivo settings [28, 35].
This data may aid current understanding of the acquisition of clinical immunity to malaria in endemic areas. Induction of antibodies to polymorphic antigens in the field upon infection with different parasite strains may be through an original antigenic sin mechanism, and individuals will most likely accumulate a strain-transcending repertoire of antibodies over time. This will also explain why clinical testing of a mono-allelic vaccine based on a polymorphic antigen in an unexposed population yields antibodies that react better with homologous than heterologous antigenic alleles  while antibodies taken after a similar trial in a malaria-endemic population react equally well with both homologous and heterologous vaccine alleles . A mixture of strain-specific and cross-strain antibodies are most likely induced in naïve individuals in the former instance while previous exposure in the latter results in a boost of responses to epitopes that are common to the vaccine and previously encountered alleles.
In summary, a mixed antigen immunization protocol is expected to elicit humoral responses similar to those elicited by a sequential immunization protocol, and by extension the response induced naturally in individuals in malaria-endemic populations. Thus the anti-AMA1 component of a natural immune response can be effectively mimicked by immunization with a cocktail of AMA1 alleles. This finding may also apply to the many other polymorphic parasite antigens that are currently undergoing clinical evaluation. Additionally, sequential exposure to different AMA1 alleles induces immunological recall of responses to previous alleles and yields functional cross-strain antibodies that are capable of optimal parasite growth inhibitions at high enough concentrations. These findings may aid current understanding of the natural acquisition of clinical immunity to malaria as well as provide fresh insight into rational vaccine design.
Acknowledgements and funding
We are grateful to Roberto Rodriguez Garcia for help with parasite AMA1 strain verification. We also thank Els Klooster for assistance with mycoplasma screening for all parasite cultures. BioGenes GmbH, Berlin, provided the adjuvant used in this study.
This work was funded by the European Malaria Vaccine Initiative (EMVI), grant number 5-2007, and the European Malaria Vaccine Development Association (EMVDA), grant number LSHP-CT-2007-037506. KAK was also supported by the Ghana Education Trust Fund. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
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