- Open Access
Plasmodium falciparum merozoite surface protein 2: epitope mapping and fine specificity of human antibody response against non-polymorphic domains
Malaria Journal volume 13, Article number: 510 (2014)
Two long synthetic peptides representing the dimorphic and constant C-terminal domains of the two allelic families of Plasmodium falciparum merozoite surface proteins 2 are considered promising malaria vaccine candidates. The aim of the current study is to characterize the immune response (epitope mapping) in naturally exposed individuals and relate immune responses to the risk of clinical malaria.
To optimize their construction, the fine specificity of human serum antibodies from donors of different age, sex and living in four distinct endemic regions was determined in ELISA by using overlapping 20 mer peptides covering the two domains. Immune purified antibodies were used in Western blot and immunofluorescence assay to recognize native parasite derivate proteins.
Immunodominant epitopes were characterized, and their distribution was similar irrespective of geographic origin, age group and gender. Acquisition of a 3D7 family and constant region-specific immune response and antibody avidity maturation occur early in life while a longer period is needed for the corresponding FC27 family response. In addition, the antibody response to individual epitopes within the 3D7 family-specific region contributes to protection from malaria infection with different statistical weight. It is also illustrated that affinity-purified antibodies against the dimorphic or constant regions recognized homologous and heterologous parasites in immunofluorescence and homologous and heterologous MSP2 and other polypeptides in Western blot.
Data from this current study may contribute to a development of MSP2 vaccine candidates based on conserved and dimorphic regions thus bypassing the complexity of vaccine development related to the polymorphism of full-length MSP2.
One strategy of malaria intervention is the development of a safe and effective blood-stage vaccine against Plasmodium falciparum[1, 2]. The complex life cycle of P. falciparum, the wide range of blood stage proteins and their extensive polymorphism provide many options for vaccine design but also render selection of the appropriate antigen(s) and vaccine development challenging. To overcome obstacles to vaccine development resulting from antigen polymorphism, this study focused only on non- or semi-polymorphic regions of promising vaccine candidates[3–7]. One of these is merozoite surface protein 2 (MSP2), a blood-stage protein that appears to be essential for viability and completion of the Plasmodium life cycle in humans[8–11]. While its function is not known, it induces specific antibodies (Abs) that are active in vitro against parasite merozoites[12–14] and are associated with protection in endemic areas.
MSP2 is a glycosylphosphatidylinositol (GPI)-anchored protein present on the merozoite surface consisting of about 200–250 amino acids, encoded by a single exon on chromosome 2. It contains conserved N- and C-terminal (C) regions flanking a highly polymorphic central repeat region. A non-repeat semi-conserved dimorphic (D) region defines the two allelic families of MSP2: 3D7 and FC27. D and C region families display low structural complexity due to the high percentage of hydrophilic residues, and are predicted and shown to represent “intrinsically unstructured regions”[4, 17]. It has been shown that specific semi-immune Ab against MSP2 protein is predominantly cytophilic IgG3, as in other blood stage proteins[4, 12, 13, 18]. These cytophilic (IgG1 and IgG3) Abs are thus thought to play an important role in antibody-mediated mechanisms of parasite clearance[19, 20].
A full-length recombinant MSP2 protein was tested in clinical trials as one of the constituents of a three-component malaria vaccine, Combination B[21, 22], containing ring-infected erythrocyte surface antigen (RESA), MSP1 and MSP2 (3D7 variant). The product was safe and partially protective. This effect was, at least in part, due to the immune response against the MSP2-3D7 allele. The 3D7-MSP2 vaccinated group had lower prevalence of parasites carrying this allelic form, while a higher incidence of morbidity episodes was associated with heterologous FC27-type infections[21–24]. These findings suggested that: i) inclusion of both allelic families in a MSP2-based vaccine should increase its efficacy, and ii) an immune response against the highly variable repeat region of MSP2 was probably not involved in protection from 3D7 parasite infection, since the 3D7 repeat present in the vaccine was found very rarely in MSP2 variants in the study area. In a recent phase I clinical trial, a recombinant vaccine candidate containing both the 3D7 and FC27 full-length proteins showed that the majority of vaccinated subjects elicited Abs that were specific for both forms of MSP2 and active in inhibiting parasite growth in antibody-dependent cellular inhibition (ADCI).
In our own investigations only D and C domains of both MSP2 allelic variants were considered, due to the high polymorphism of the central region of MSP2, while the non-polymorphic N-terminal region was excluded because it favours amyloid fibril formation within the MSP2 molecule which potentially leads to regulatory issues. The choice of D and C domains was motivated by the finding showing that the Abs against the 3D7 family specific and constant domain (D + C) was associated with protection from clinical malaria and were active in ADCI[4, 12, 23]. The present study used overlapping 20-mer peptides and donors from different endemic areas, varying by age and sex to identify fragments within the D and C regions with promising vaccine potential.
The schematic structure and full-length sequence alignment of the two allelic families of MSP2 are shown respectively in Figures 1A and1B. All peptides were synthesized at the Department of Biochemistry, University of Lausanne, Switzerland, using an Applied Biosystem 431A instrument (Foster City, CA, USA) and Fmoc chemistry and capping of the unreactive peptide chains with acetic anhydride at each cycle. The purity of each peptide (>80%) was determined using analytical C18 HPLC and mass spectroscopy. Lyophilized peptides were dissolved in phosphate buffered saline (PBS (Gibco® Invitrogen™)) at a concentration of 1 mg/ml. Different LSPs derivate from both allelic families of MSP2 are represented in Additional file1. Overlapping 20-mer peptides (overlapping by ten amino acids) were synthesized by using the MultiRespep Synthesizer (Bioanalytical Instrument, Intavis AG). Thus, 12 20-mer peptides (P11-P22) and eight 20-mer peptides (P23-P30) covered, respectively, 3D7 and FC27-MSP2 D + C region. Thus, the 3D7 20 mers P20, P21 and P22 are similar to the FC27 20 mers P28, P29 and P30. Peptides P19 (from 3D7 family) and P27 (from FC27 family) contained the eight last aa of the D regions, respectively, plus the 12 first aa of their C region (Figure 1C).
Human sera or plasma samples were collected during the malaria transmission season in each endemic area. Adult donors were from Burkina Faso (BF), Papua New Guinea (PNG), Tanzania (TZ), Nigeria (NG). Donors from Mali were categorized into three age groups (≤five years, six to 14 years and ≥15 years).
For the analysis of association of antibody responses with protection two hundred and eighty sera from children of one to five years of age in the village of Idete in Tanzania were available. These children formed the placebo group of an SPf66 vaccine efficacy trial. All illness episodes in these children reporting to the local health centre during a one-year follow-up after collection of these sera were recorded, and malaria slides prepared for determination of parasite positivity and densities. For analysis of the relationship of protection to antibody levels a clinical malaria episode was defined as measured fever (> or = 37.5 degrees C) and parasite density > 20,000/microL. This was the same definition as was used in the original trial. Research and ethical clearance was granted by the Tanzanian Commission for Science and Technology (UTAFITI NSR/RCA 90).
Sera from Swiss naive donors (12 to 13 individual donors) who had no malaria history were used as a negative control. Blood was taken by venipuncture into tubes containing EDTA according to the ethical clearances of each country. Research carried out on humans was conducted in compliance with the Helsinki Declaration. Some donors with high Ab titres were selected in single or pooled to purify Abs (pAbs) reactive to D, C and D + C fragments of the two allelic families of MSP2, and 3D7-D + 8aaC LSP of 3D7 family.
Affinity purification of human polyclonal antibodies
Reactive Abs to FC27-D + C, 3D7-D + 8aa C, 3D7-D, FC27-D and C LSPs were purified from ELISA positive plasma from BF, PNG, NG adults and different age groups from Mali using affinity chromatography as previously described. Briefly, 5 mg of peptides were added to 1 ml of activated sepharose and processed according to manufacture instructions.
Enzyme-linked immunosorbent assay
For enzyme-linked immunosorbent assay (ELISA), antigen concentration for coating 96-well flat plates (BD Biosciences) was 1 μg/ml for peptides longer than 40 residues, and 5 μg/ml for peptides shorter or equal to 40 residues. As previously described[5, 28, 29], plates were coated overnight (O/N) with 50 μl of peptide at the appropriate concentration in PBS and then blocked for one hour at room temperature (RT) in PBS containing 5% non-fat milk powder. Test was considered positive if the sample OD mean was ≥ OD mean + 3 SD of negative controls (non-exposed Swiss donors) or if the ratio of sample OD mean divided by OD mean of negative controls was ≥2. Each sample was tested in duplicate.
A native protein is characterized by its folded structure; increasing the chaotropic characteristics of solvent leads to denaturation. Guanidine chloride (GdCl, Merck KGaA, Darmstadt, Germany) is one of the general protein denaturants leading to protein unfolding[30, 31]. Briefly, for measuring Ab avidity by ELISA, different concentrations of GdCl (8 M, 4 M, 2 M, 1 M and 0 M) were mixed with plasma for 30 min before transferring the mixture into peptide-coated plates. Relative avidity was determined by the concentration of GdCl needed to obtain 50% of the OD value in the absence of GdHCl. Thus samples with OD at 1 M GdHCl higher or equal to 50% of the OD in the absence of GdHCl (0 M) were considered having higher avidity than those with less than 50% of the OD in the absence of GdHCl.
Immunofluorescence and Western Blot
Immunofluorescence assay (IFA) was performed on blood smear slides containing at least 5% schizontes of 3D7 and FC27 P. falciparum cultures and Western blot (WB) were performed using reduced 3D7 and FC27 parasite lysates[5, 28].
Pearson’s Chi-square or Fisher’s exact tests were used to assess association between categorical variables and ANOVA tests (GraphPad Prism, version 5.00) were used to test differences between groups in antibody levels. The relationship between antibody-levels measured in ELISA and the incidence of clinical malaria in the Tanzanian children was evaluated by Kaplan Meier analysis, including tests of significance using log rank chi-square tests. The effects were tested both with age-adjustment, and without adjustment for age.
Recognition of individual domains by human sera and delineation of B cell epitopes
The intrinsically unstructured D and C offers an ideal opportunity to study the fine specificity of MSP2-reactive human Abs using long and/or short overlapping peptides. The lengths of different LSPs covering D and C regions of the two allelic family regions are showed in Additional file1. Purified Abs (pAbs) reactive with D + C of each allelic family (obtained from Nigerian adult pooled plasma) and tested in ELISA showed that each dimorphic derivate and C region LSP was well recognized. However, 3D7-D LSP was better recognized than that of C region while the contrary was observed for FC27-D LSP, respectively (Figure 2A and B). Cytophilic IgG1 and IgG3 were the most prevalent subclasses recognizing the 3D7-D and C LSP while recognition of FC27-D LSP was mainly associated with IgG1 (Additional file2).
In order to study the fine specificity of the antibody response outlined above, 20-mer peptides (overlapping by 10 aa) covering the two allelic regions, D and C regions of MSP2 were tested.
First, sera of adults living in four different endemic regions were tested in ELISA to see if MSP2 20 mers were equally recognized. The prevalence (% positive samples in ELISA test), OD and SD of Ab responses for each peptide are shown in Table 1. The most frequently recognized 20 mers in the 3D7-D region were P13, which was recognized by 67 and 51% of donors from PNG and TZ, respectively, and P13/16, recognized by 46% of the donors from Mali, as well as P17 recognized by 69% from BF. For the FC27-D region, the most prevalent 20 mers were P23 with 48% in PNG, P25 with 45 and 18%, respectively in BF and in Mali, and P26 with 51% in TZ. For the C region, P29 appeared the most prevalent in PNG (50%), BF (39%) and in Mali (13%) while in TZ the most frequent was P30 with 43% (Table 1). Overall, considering the overall prevalence in the four areas, P13 (51%) and P16 (48%) were the most prevalent for the 3D7-D; P23 (28%) and P25 (31%) were for the FC27-D, and P29 and P30 (30%) for C-region (Table 1). However, the frequency of recognition of these commonly seen 20 mers, except for P13 (immunodominant epitopes) differed significantly among the four endemic areas (p <0.05). At all sites, 3D7-D was more frequently recognized than FC27-D or the C region while the frequency was similar among FC27-D and C regions (Table 1).
These data showed that all 20-mer peptides were antigenic and led to the delineation of immunodominant MSP2 epitopes in endemic areas tested.
Fine specificity of D and C region recognition in different age groups
Epitope mapping was extended to donors divided into three age groups (children ≤ five years, adolescents six to 14 years and adults ≥15 years) living in Mali. Samples were collected during the malaria transmission season. The prevalence of the most recognized 20 mers of the 3D7-D and C domains did not depend on the age of donors (Table 2). In contrast, for the FC27-D region, acquisition of immune responses against the 20 mers increased significantly with age, in particular, there were significant differences between the children and adults children (Table 2).
In the context of this evidence that immune responses against the D and C regions are acquired early in individuals exposed to malaria, the detailed age profile of immune response acquisition in the earlier life of donors was examined in the 186 sera from Tanzanian children of different ages (one to five years). Immune responses against most of peptides increased with age until two to three years old, but tended to decrease in four years old children. Thereafter Ab responses remained stable or increased again (Figure 3A). A similar pattern of Ab responses was observed also for LSPs covering D + C region of the two MSP2 allelic families, the C region alone (Figure 3B). To determine if this was a general phenomenon, other unstructured LSPs derived from a blood or pre-erythrocytic stage proteins, PFF0165c, P27A, MR252, exported proteins Pf EXP1, MR127B[32, 33], and N-terminal circumsporozoite (CS) protein fragments (MR48 and MR48A) (Additional file1) were tested in ELISA. Interestingly, only Ab responses against LSPs from MSP2 increased with age until two to three years followed by a modest decrease in four years old while those to EXP1, CS and P27A LSPs tended to increase or remain stable at this age (Figure 3B).
Relative avidity of antibodies to D- and C-LSPs and their immunodominant epitopes in different age groups
Antibody avidity is one of the parameters used to determine the maturation of an immune response[35–39]. Relative avidity of Abs reactive to different fragments of MSP2 and their 20 mers was determined by using different concentrations of GdCl at a fixed serum dilution (1:200) in ELISA (data not shown). Eleven plasma samples per age group from Malian donors that gave the highest OD in ELISA against D and C were tested. By considering the OD value curve at different concentrations of the GdCl (i.e., the number of samples with OD at 1 M GdCl higher than 50% of the OD at no GdCl), the relative avidity between the 3D7-D LSP and its specific Ab appeared similar for different age groups as shown in Additional file3A. In contrast, relative avidity for FC27-D specific Abs was low in children and increased with age (children < adolescents < adults, (children versus adults, p <0.05 (*)) (Additional file3B)) whereas, relative avidity of Abs for the C region was higher in children compared to adolescents and adults (p <0.05 (*) and P ≤ 0.001 (**), respectively) (Additional file3C). These results are consistent with those obtained above regarding age dependency of immune responses.
Association of the immune antibody response elicited against individual 3D7-D 20 mers in children with protection from malaria
It has been shown earlier that the antibody response to 3D7 D + C but not FC27 D + C region is associated with protection from malaria clinical malaria. In addition, the antibody response to 3D7-D + 8aa C-terminal conserved residues was also associated with protection in the Tanzanian children cohort. This analysis was then extended to 3D7-D LSP and its corresponding 20 mers in the same Tanzanian children. The relationship between malaria morbidity and antibody OD at baseline was determined for each peptide. Peptides P11, P12, P13 and P16 were associated with the highest probability in protection (Figure 4A). Except for P11, the peptides P12, P13 and P16 were among the immunodominant epitopes of 3D7-D as shown above in Table 1. These epitopes showed a slightly increased or similar association with protection compared to the reference LSP of 3D7-D. However, their association with protection was not statistically significant (p >0.05) (Figure 4A).Since peptides P11, P12 and P13 showed the strongest association with protection, a longer peptide, called P2604 (111–150; 40 aa) containing the three sequences was synthesized. ELISA test performed in the cohort of Tanzanian children indeed showed an increased recognition P2604, but the association with protection did not reach a significance level (Figure 4B and C) for either peptide P2604 or D.
Cross-reaction of D- and C-LSP purified antibodies in WB and IFA
As reported previously, 3D7-D and FC27-D human reactive Abs inhibited heterologous parasite growth as determined in ADCI and recognized heterologous MSP2 recombinant proteins in ELISA. To confirm these findings, analysis was extended using 3D7-D, FC27-D and C LSP affinity purified Abs from single adult BF donors. In WB, the FC27-D pAbs recognized only family-specific proteins whereas 3D7-D pAbs recognized both 3D7 and FC27 P. falciparum-derived proteins (Figure 5A and B). Cross-reactive bands observed were depending on serum donor (Figure 5A). As expected, the C region-reactive pAbs recognized both 3D7 and FC27-strain derived merozoite proteins (Figure 5C). Note that MSP2 is localized between 55–35 kD included. Additionally, pAbs from plasma pools of donors of different ages and single adult C-reactive pAbs were used to perform IFA on both of the 3D7 and FC27 schizonts. All of the 3D7-D specific pAbs recognized both homologous (3D7) and heterologous (FC27) merozoites confirming the cross-binding reaction (Additional file4A and B). Due to the low level of antibody titre against the FC27-D region found in children and adolescents, the reverse experiment could not be performed. As for WB, C region-reactive pAbs recognized both 3D7 and FC27 parasites in IFA (Additional file4C).
The aim of the current studies was the delineation of immunodominant and protective D and C epitopes in individuals living in different malaria-endemic areas in order to develop more effective MSP2-based universal vaccines either as a single candidate or in combination with other antigens.
Here, the first observation was that the immunodominant 20-mer epitopes contained in each single MSP2 domain (P13, P15/16 for 3D7-D; P23, P25/P26 for FC27 and P29/P30 for C) are in part conserved in the four endemic areas analysed (Table 1). Differences in the level and specificity of serum or affinity purified antibodies of single individuals are observed and may depend on the history of infections by different P. falciparum variant strains and/or on the genetic diversity of donors[16, 40, 41]. In general, recognition of the 3D7-D major epitopes is more prevalent than that observed for FC27-D and C regions (Table 1) in agreement with data shown by other groups either for the full-length proteins or fragments thereof[3, 4, 7]. In addition, Ab responses against D or C region of each MSP2 allelic family and individual 20 mers were similar in male and female populations living in the same endemic area (Additional file5), thus facilitating the development of universal MSP2-based vaccines.
The acquisition of an optimal response as judged by ELISA is obtained early in life (age two to three years) for the 3D7-D and its 20 mers as seen for several pre-erythrocytic and erythrocytic antigens (Figure 3A, B). This is further confirmed when the relative avidity of the Ab response in the three age groups was determined. In contrast, for the FC27-D region, as observed for the magnitude of the response, the apparent avidity of Ab is low in the children, and increases with age (Additional file3). Together, these data confirm that the response to 3D7 MSP2 matures earlier in life compared to that to FC27 MSP2, most likely due to a higher rate of infection by 3D7-family parasites[7, 42, 43]. In addition, the relative avidity of Abs against C region appeared strongest in children compared to that shown in adolescent and adult groups (Additional file3). This confirms observations from other groups who showed that the positive Ab responses to C-region were observed only in children and not in adults[44–46].
Antibodies to P. falciparum MSP2 antigens belong predominantly to the cytophilic and complement-fixing subclasses IgG1 and IgG3, and have been shown to be associated with protection from clinical malaria in immune adults[13, 47, 48]. This study confirmed that IgG1 and IgG3 are the most relevant subclasses associated with MSP2 LSP recognition in adults, but also in adolescent and children (Additional file2).
As described before[10, 14, 49, 50], 3D7- and FC27-D pAbs recognize the heterologous RecMSP2 (recombinant MSP2 protein) in ELISA and here parasite-derived proteins in WB and IFA (Figure 5, Additional file4). The cross-binding between the two allelic MSP2 families occurred only between MSP2 full-length recombinant proteins or parasite-derived proteins but not for LSP. Moreover, the cross binding was strictly dependent on the donors, suggesting a possible influence of parasite infections experienced by single donors and/or individual genetic differences. Cross-binding with higher molecular weight protein(s) was also observed using mouse sera or monoclonal antibodies derived by mouse immunization with MSP2 peptides. Bio-informatic analysis indicates a number of possible cross-reacting proteins (Additional file6), and proteomic experiments are needed to identify them. As expected, C region specific pAbs recognized both allelic parasite-derived proteins, further justifying its inclusion in a MSP2 vaccine development. The extensive cross-reaction discussed above may be beneficial for the acquisition of a protective immune response.
Finally, the association of the Abs response to 3D7-D region and its epitopes with protection from clinical malaria was not statistically significant (p >0.05) but showed a diverse degree of probability, with P11, P12 and P13 mers having the highest probability. Analysis of the fragment P2604 containing the P11, P12 and P13 sequences led to increased recognition by Ab in different age groups (compared to single constitutive 20 mers) but was not associated with protection. Similarly, repeat testing of the same cohort for the antigen D +8aaC gave smaller estimates of relative risk, suggesting that the promising result previously obtained may well be a chance finding. Thus, testing of other paediatric cohorts is needed to assess the impact of D + 8aaC in protection.
World Health Organization: Malaria. http://www.who.int/topics/malaria/en/ 2011
World Health Organization: World Malaria Report. 2011, http://www.who.int/malaria/world_malaria_report_2011/en/index.html 2011
Flueck C, Smith T, Beck HP, Irion A, Betuela I, Alpers MP, Anders R, Saul A, Genton B, Felger I: Strain-specific humoral response to a polymorphic malaria vaccine. Infect Immun. 2004, 72: 6300-6305. 10.1128/IAI.72.11.6300-6305.2004.
Flueck C, Frank G, Smith T, Jafarshad A, Nebie I, Sirima SB, Olugbile S, Alonso P, Tanner M, Druilhe P, Felger I, Corradin G: Evaluation of two long synthetic merozoite surface protein 2 peptides as malaria vaccine candidates. Vaccine. 2009, 27: 2653-2661. 10.1016/j.vaccine.2009.02.081.
Olugbile S, Kulangara C, Bang G, Bertholet S, Suzarte E, Villard V, Frank G, Audran R, Razaname A, Nebie I, Awobusuyi O, Spertini F, Kajava AV, Felger I, Druilhe P, Corradin G: Vaccine potentials of an intrinsically unstructured fragment derived from the blood stage associated Plasmodium falciparum protein PFF0165c. Infect Immun. 2009, 77: 5701-5709. 10.1128/IAI.00652-09.
Theisen M, Dodoo D, Toure-Balde A, Soe S, Corradin G, Koram KK, Kurtzhals JA, Hviid L, Theander T, Akanmori B, Ndiaye M, Druilhe P: Selection of glutamate-rich protein long synthetic peptides for vaccine development: antigenicity and relationship with clinical protection and immunogenicity. Infect Immun. 2001, 69: 5223-5229. 10.1128/IAI.69.9.5223-5229.2001.
Felger I, Tavul L, Kabintik S, Marshall V, Genton B, Alpers M, Beck HP: Plasmodium falciparum: extensive polymorphism in merozoite surface antigen 2 alleles in an area with endemic malaria in Papua New Guinea. Exp Parasitol. 1994, 79: 06-116.
Carvalho LJ, Daniel-Ribeiro CT, Goto H: Malaria vaccine: candidate antigens, mechanism, constraints. Scand J Immunol. 2002, 56: 327-343. 10.1046/j.1365-3083.2002.01160.x.
Cowman AF, Baldi DL, Healer J, Mills KE, O’Donnell RA, Reed MB: Functional analysis of proteins involved in Plasmodium falciparum merozoite invasion of red blood cells. FEBS Lett. 2000, 476: 84-88. 10.1016/S0014-5793(00)01703-8.
Epping RJ, Goldstone SD, Ingram LT, Upcroft JA, Ramasamy R, Cooper JA: An epitope recognised by inhibitory monoclonal antibodies that react with a 51 kilodalton merozoite surface antigen in Plasmodium falciparum. Mol Biochem Parasitol. 1988, 28: 1-10. 10.1016/0166-6851(88)90173-9.
Ramasamy R, Jones G, Lord R: Characterisation of an inhibitory monoclonal antibody-defined epitope on a malaria vaccine candidate antigen. Immunol Lett. 1990, 23: 305-309. 10.1016/0165-2478(90)90077-4.
Taylor RR, Smith DB, Robinson VJ, McBride JS, Riley EM: Human antibody response to Plasmodium falciparum merozoite surface protein 2 is serogroup specific and predominantly of the immunoglobulin G3 subclass. Infect Immun. 1995, 63: 4382-4388.
Metzger WG, Okenu DM, Cavanagh DR, Robinson JV, Bojang KA, Weiss HA, McBride JS, Greenwood BM, Conway DJ: Serum IgG3 to the Plasmodium falciparum merozoite surface protein 2 is strongly associated with a reduced prospective risk of malaria. Parasite Immunol. 2003, 25: 307-312. 10.1046/j.1365-3024.2003.00636.x.
Stubbs J, Olugbile S, Saidou B, Simpore J, Corradin G, Lanzavecchia A: Strain-transcending Fc-dependent killing of Plasmodium falciparum by merozoite surface protein 2 allele-specific human antibodies. Infect Immun. 2011, 79: 1143-1152. 10.1128/IAI.01034-10.
Anders RF, Smythe JA: Polymorphic antigens in Plasmodium falciparum. Blood. 1989, 74: 1865-1875.
Felger I, Marshal VM, Reeder JC, Hunt JA, Mgone CS, Beck HP: Sequence diversity and molecular evolution of the merozoite surface antigen 2 of Plasmodium falciparum. J Mol Evol. 1997, 45: 154-160. 10.1007/PL00006215.
Wright PE, Dyson JH: Intrinsically unstructured proteins: re-assessing the protein structure-function paradigm. J Mol Biol. 1999, 293: 321-331. 10.1006/jmbi.1999.3110.
Taylor RR, Allen SJ, Greenwood BM, Riley EM: IgG3 antibodies to Plasmodium falciparum merozoite surface protein 2 (MSP2): increasing prevalence with age and association with clinical immunity to malaria. Am J Trop Med Hyg. 1998, 58: 406-413.
Tebo AE, Kremsner PG, Luty AJ: Plasmodium falciparum: a major role for IgG3 in antibody-dependent monocyte-mediated cellular inhibition of parasite growth in vitro. Exp Parasitol. 2001, 98: 20-28. 10.1006/expr.2001.4619.
Bouharoun-Tayoun H, Oeuvray C, Lunel F, Druilhe P: Mechanisms underlying the monocyte-mediated antibody-dependent killing of Plasmodium falciparum asexual blood stages. J Exp Med. 1995, 182: 409-418. 10.1084/jem.182.2.409.
Genton B, Al-Yaman F, Anders R, Saul A, Brown G, Pye D, Irving DO, Briggs WR, Mai A, Ginny M, Adiguma T, Rare L, Giddy A, Reber-Liske R, Stuerchler D: Safety and immunogenicity of a three-component blood-stage malaria vaccine in adults living in an endemic area of Papua New Guinea. Vaccine. 2000, 18: 2504-2511. 10.1016/S0264-410X(00)00036-0.
Saul A, Lawrence G, Smillie A, Rzepczyk CM, Reed C, Taylor D, Anderson K, Stowers A, Kemp R, Allworth A, Anders RF, Brown GV, Pye D, Schoofs P, Irving DO, Dyer SL, Woodrow GC, Briggs WR, Reber R, Stürchler D: Human phase I vaccine trials of 3 recombinant asexual stage malaria antigens with Montanide ISA720 adjuvant. Vaccine. 1999, 17: 3145-3159. 10.1016/S0264-410X(99)00175-9.
Genton B, Betuela I, Felger I, Al-Yaman F, Anders RF, Saul A, Rare L, Baisor M, Lorry K, Brown GV, Pye D, Irving DO, Smith TA, Beck HP, Alpers MP: A recombinant blood-stage malaria vaccine reduces Plasmodium falciparum density and exerts selective pressure on parasite populations in a phase 1–2b trial in Papua New Guinea. J Infect Dis. 2002, 185: 820-7. 10.1086/339342.
Genton B, Al-Yaman F, Betuela I, Anders RF, Saul A, Baea K, Mellombo M, Taraika J, Brown GV, Pye D, Irving DO, Felger I, Beck HP, Smith TA, Alpers MP: Safety and immunogenicity of a three-component blood-stage malaria vaccine (MSP1, MSP2, RESA) against Plasmodium falciparum in Papua New Guinean children. Vaccine. 2003, 22: 30-41. 10.1016/S0264-410X(03)00536-X.
McCarthy JS, Marjason J, Elliott S, Fahey P, Bang G, Malkin E, Tierney E, Aked-Hurditch H, Adda C, Cross N, Richards JS, Fowkes FJ, Boyle MJ, Long C, Druilhe P, Beeson JG, Anders RF: A phase 1 trial of MSP2-C1, a blood-stage malaria vaccine containing 2 isoforms of MSP2 formulated with montanide ISA 720. PLoS One. 2011, 6: e2443-
Adda CG, Murphy VJ, Sunde M, Waddington LJ, Schloegel J, Talbo GH, Vingas K, Kienzle V, Masciantonio R, Howlett GJ, Hodder AN, Foley M, Anders RF: Plasmodium falciparum merozoite surface protein 2 is unstructured and forms amyloid-like fibrils. Mol Biochem Parasitol. 2009, 166: 159-171. 10.1016/j.molbiopara.2009.03.012.
Alonso PL, Smith T, Schellenberg JR, Masanja H, Mwankusye S, Urassa H, Bastos de Azevedo I, Chongela J, Kobero S, Menendez C: Randomised trial of efficacy of SPf66 vaccine against Plasmodium falciparum malaria in children in southern Tanzania. Lancet. 1994, 344: 1175-1181. 10.1016/S0140-6736(94)90505-3.
Villard V, Agak GW, Frank G, Jafarshad A, Servis C, Nébié I, Sirima SB, Felger I, Arevalo-Herrera M, Herrera S, Heitz F, Bäcker V, Druilhe P, Kajava AV, Corradin G: Rapid identification of malaria vaccine candidates based on α-helical coiled coil protein motif. PLoS One. 2007, 2: e645-10.1371/journal.pone.0000645.
Agak GW, Bejon P, Fegan G, Gicheru N, Villard V, Kajava AV, Marsh K, Corradin G: Longitudinal analyses of immune responses to Plasmodium falciparum derived peptides corresponding to novel blood stage antigens in coastal Kenya. Vaccine. 2008, 26: 1963-1971. 10.1016/j.vaccine.2008.02.020.
Nozaki Y, Tanford C: Proteins as random coils. II. Hydrogen ion titration curve of ribonuclease in 6 M guanidine hydrochloride. J Am Chem Soc. 1967, 89: 736-742. 10.1021/ja00980a002.
Garcia-Mira MM, Sanchez-Ruiz JM: pH Corrections and Protein Ionization in Water/Guanidinium Chloride. Biophys J. 2001, 81: 3489-3502. 10.1016/S0006-3495(01)75980-2.
Sanchez GI, Rogers WO, Mellouk S, Hoffman SL: Plasmodium falciparum: exported protein-1, a blood stage antigen, is expressed in liver stage parasites. Exp Parasitol. 1994, 79: 59-62. 10.1006/expr.1994.1060.
Meraldi V, Nebié I, Tiono AB, Diallo D, Sanogo E, Theisen M, Druilhe P, Corradin G, Moret R, Sirima BS: Natural antibody response to Plasmodium falciparum Exp-1, MSP-3 and GLURP long synthetic peptides and association with protection. Parasite Immunol. 2004, 26: 265-272. 10.1111/j.0141-9838.2004.00705.x.
Bongfen SE, Ntsama PM, Offner S, Smith T, Felger I, Tanner M, Alonso P, Nebie I, Romero JF, Silvie O, Torgler R, Corradin G: The N-terminal domain of Plasmodium falciparum circumsporozoite protein represents a target of protective immunity. Vaccine. 2009, 27: 328-335. 10.1016/j.vaccine.2008.09.097.
Ferreira MU, Kimura EA, De Souza JM, Katzin AM: The isotype composition and avidity of naturally acquired anti-Plasmodium falciparum antibodies: differential patterns in clinically immune Africans and Amazonian patients. Am J Trop Med Hyg. 1996, 55: 315-23.
Leoratti FM, Durlacher RR, Lacerda MV, Alecrim MG, Ferreira AW, Sanchez MC, Moraes SL: Pattern of humoral immune response to Plasmodium falciparum blood stages in individuals presenting different clinical expressions of malaria. Malar J. 2008, 7: 186-10.1186/1475-2875-7-186.
Hedman K, Lappalainen M, Söderlund M, Hedman L: Avidity of IgG in serodiagnosis of infectious diseases. Rev Med Microbiol. 1993, 4: 123-129. 10.1097/00013542-199307000-00001.
Thomas HI, Wilson S, O’Toole CM, Lister CM, Saeed AM, Watkins RP, Morgan-Capner P: Differential maturation of avidity of IgG antibodies to gp41, p24 and p17 following infection with HIV-1. Clin Exp Immunol. 1996, 103: 185-191. 10.1046/j.1365-2249.1996.951642.x.
Marcipar SI, Risso GM, Silber MA, Revelli S, Marcipar JA: Antibody maturation in Trypanosoma cruzi-infected rats. Clin Diagn Lab Immunol. 2001, 8: 802-805.
Franks S, Baton L, Tetteh K, Tongren E, Dewin D, Akanmori BD, Koram KA, Ranford-Cartwright L, Riley EM: Genetic diversity and antigenic polymorphism in Plasmodium falciparum: extensive serological cross-reactivity between allelic variants of merozoite surface protein 2. Infect Immun. 2003, 71: 3485-3495. 10.1128/IAI.71.6.3485-3495.2003.
Felger I, Steiger S, Hatz C, Smith T, Beck HP: Antigenic cross-reactivity between different alleles of the Plasmodium falciparum merozoite surface protein 2. Parasite Immunol. 2003, 25: 531-543. 10.1111/j.0141-9838.2004.00664.x.
Falk N, Maire N, Sama W, Owusu-Agyei S, Smith T, Beck HP, Felger I: Comparison of PCR-RFLP and Genescan-based genotyping for analyzing infection dynamics of Plasmodium falciparum. Am J Trop Med Hyg. 2006, 74: 944-950.
Henning L, Schellenberg D, Smith T, Henning D, Alonso P, Tanner M, Mshinda H, Beck HP, Felger I: A prospective study of Plasmodium falciparum multiplicity of infection and morbidity in Tanzanian children. Trans R Soc Trop Med Hyg. 2004, 98: 687-694. 10.1016/j.trstmh.2004.03.010.
Lawrence N, Stowers A, Mann V, Taylor D, Saul A: Recombinant chimeric proteins generated from conserved regions of Plasmodium falciparum merozoite surface protein 2 generate antiparasite humoral responses in mice. Parasite Immunol. 2000, 22: 211-221. 10.1046/j.1365-3024.2000.00293.x.
Thomas AW, Carr DA, Carter JM, Lyon JA: Sequence comparison of allelic forms of the Plasmodium falciparum merozoite surface antigen MSA2. Mol Biochem Parasitol. 1990, 43: 211-220. 10.1016/0166-6851(90)90146-D.
Stowers A, Taylor D, Prescott N, Cheng Q, Cooper J, Saul A: Assessment of the humoral immune response against Plasmodium falciparum rhoptry-associated proteins 1 and 2. Infect Immun. 1997, 65: 2329-2338.
Osier FH, Murungi LM, Fegan G, Tuju J, Tetteh KK, Bull PC, Conway DJ, Marsh K: Allele-specific antibodies to Plasmodium falciparum merozoite surface protein-2 and protection against clinical malaria. Parasite Immunol. 2010, 32: 193-201. 10.1111/j.1365-3024.2009.01178.x.
Bouharoun-Tayoun H, Druilhe P: Plasmodium falciparum malaria: evidence for an isotype imbalance which may be responsible for delayed acquisition of protective immunity. Infect Immun. 1992, 60: 1473-1481.
Fenton B, Clark JT, Khan CM, Robinson JV, Walliker D, Ridley R, Scaife JG, McBride JS: Structural and antigenic polymorphism of the 35- to 48-kilodalton merozoite surface antigen (MSA-2) of the malaria parasite Plasmodium falciparum. Mol Cell Biol. 1991, 11: 963-971.
Saul A, Lord R, Jones G, Geysen HM, Gale J, Mollard R: Cross-reactivity of antibody against an epitope of the Plasmodium falciparum second merozoite surface antigen. Parasite Immunol. 1989, 11: 593-601. 10.1111/j.1365-3024.1989.tb00923.x.
Plasmo DB: The Plasmodium genome resource. http://plasmodb.org 2014, Version 12.0
This work has been supported by the European Vaccine Initiative and EC LSHP-CT-2007-037506 grants. Thank you to Prof Robin Anders for providing of the two recombinant MSP2 proteins and Dr Alice Koumaré of the Centre National de Transfusion Sanguine in Ouagadougou, Burkina Faso for providing immune plasma.
The authors have declared that they have no competing interests.
SB, SO, IF, FS, and GC designed the study; SB, SO, AD, and GF conducted the experiments and were involved in data analysis with supervision from IF, FS and GC; CS and GC were responsible for peptide synthesis, purification and characterization; SO, MD, RM, IN, IF, and MT provided the samples for analysis; AK provided the bio-informatic analysis of sequence comparison; TS provided the analysis of association with protection. All authors contributed to writing the manuscript. All authors read and approved the final version.
Electronic supplementary material
Additional file 1: Sequences of different long synthetic peptides. The bold and underlined sequences correspond to the common C-terminal region sequence of MSP2-3D7 and FC27 families. 3D7 dimorphic derivate LSPs are 3D7-D (88 aa), 3D7-D-M4 (73 aa) and 3D7-D-MR274 (60 aa). D + C is sequence derivate from dimorphic of each family plus the C region. Note that M and MR plus different number represent only peptide code given during synthesis. Sequences of LSPs derivate from Pf EXP1 (MR127B), PFF0165C (MR252 or P27A) and P. falciparum circumsporozoite: Pf CS (MR48, MR48A from N-terminal) are also represented. (DOC 40 KB)
Additional file 2: Isotyping of IgG against D and C domain LSPs of the two allelic families of MSP2. D and C fragments of the two MSP2 allelic families were used to perform ELISA in order to define the subclass of total IgG. Individual plasma samples from children (N = 12), adolescents (N = 13), and adults (N = 14) living in Mali were used at a dilution of 1/200. ELISA was considered positive if mean of Ab OD of test sample with considered IgG subtype was more than mean OD + 3SD of negative control sera (N: 12). Percentage of positive sera for IgG1, IgG2, IgG3 and IgG4 against each region of MSP2 was thus determined. (PDF 266 KB)
Additional file 3: Determination of relative age-specific antibody avidity against D and C regions. Plasma from different age groups (children, adolescents and adults from Mali, 11 sample per age group) that elicited high Ab responses in ELISA were mixed with different concentrations of GdCl (0 to 8 M) for 30–45 minutes before transfer to ELISA plates containing corresponding peptide. A, B and C represent respectively, the relative Ab avidity to 3D7-D, FC27-D and C region LSPs. The p values show statistic difference (Fisher’s exact test) between two age groups. ns: not statistically significant, *: p < 0.05 and **: p ≤ 0.001. (PDF 98 KB)
Additional file 4: 3D7-D and C LSP purified antibodies recognized merozoite proteins derived from the two allelic family parasites. Immunofluorescence staining of malaria-infected erythrocytes was performed with age specific 3D7-D (A, B) respectively y, 3D7 and FC27 strain merozoites, and C-terminal reactive pAbs (C). The age reactive pAbs specific to 3D7-D and C were obtained from age-pooled plasma (A and B), respectively and single BF plasma (C), and used at a dilution of 1/100. Nucleus stained with DAPI (in blue) and transmission picture of the infected red blood cell (DIC). (PDF 296 KB)
Additional file 5: D and C epitope prevalence of the two allelic MSP2 according to the gender of donors. Plasma of Malian donors (regardless of age): females (F, N = 57) and males (M, N = 50) were collected during the malaria season transmission and used at dilution 1/200 to perform direct ELISA on 20 mers covering the two domains of the two MSP2 allelic families. Sample was considered positive responder if ratio of mean Ab OD/mean OD of negative control was equal to or more than 2. The p value was calculated from Fisher’s exact test that compares variation between the two sexes for each peptide (n = number;%: percent of positive donors). N = total number of donor from each sex. (DOC 66 KB)
Additional file 6: Similar shared sequences between the two allelic families of MSP2. Similar possible and shared sequences are presented here in order to explain the cross-binding occurred between the two allelic families. For this purpose, dimorphic sequences of each MSP2 allelic family were matched with those representing the heterologous family. A and B represent, respectively, sequences of FC27 and 3D7 dimorphic matched with their own and heterologous sequences, whereas C shows matching of common C-terminal sequences with the two allelic regions (minimal epitope is four amino acids). Upper case letter indicates the same amino acids; lower case letter represents the different amino acids. All data were generated from PlasmoDB database. (DOC 204 KB)
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Balam, S., Olugbile, S., Servis, C. et al. Plasmodium falciparum merozoite surface protein 2: epitope mapping and fine specificity of human antibody response against non-polymorphic domains. Malar J 13, 510 (2014) doi:10.1186/1475-2875-13-510
- Plasmodium falciparum
- Dimorphic regions
- C-terminal region
- Epitope mapping
- Fine specificity