Skip to main content
PMC home page
eLife logoLink to eLife
. 2018 Jun 19;7:e35213. doi: 10.7554/eLife.35213

Synergy in anti-malarial pre-erythrocytic and transmission-blocking antibodies is achieved by reducing parasite density

Ellie Sherrard-Smith 1,†,, Katarzyna A Sala 2,, Michael Betancourt 3, Leanna M Upton 2, Fiona Angrisano 2, Merribeth J Morin 4, Azra C Ghani 1,, Thomas S Churcher 1,, Andrew M Blagborough 2,
Editor: Urszula Krzych5
PMCID: PMC6008048  PMID: 29914622

Abstract

Anti-malarial pre-erythrocytic vaccines (PEV) target transmission by inhibiting human infection but are currently partially protective. It has been posited, but never demonstrated, that co-administering transmission-blocking vaccines (TBV) would enhance malaria control. We hypothesized a mechanism that TBV could reduce parasite density in the mosquito salivary glands, thereby enhancing PEV efficacy. This was tested using a multigenerational population assay, passaging Plasmodium berghei to Anopheles stephensi mosquitoes. A combined efficacy of 90.8% (86.7–94.2%) was observed in the PEV +TBV antibody group, higher than the estimated efficacy of 83.3% (95% CrI 79.1–87.0%) if the two antibodies acted independently. Higher PEV efficacy at lower mosquito parasite loads was observed, comprising the first direct evidence that co-administering anti-sporozoite and anti-transmission interventions act synergistically, enhancing PEV efficacy across a range of TBV doses and transmission intensities. Combining partially effective vaccines of differing anti-parasitic classes is a pragmatic, powerful way to accelerate malaria elimination efforts.

Research organism: Mouse, Other

eLife digest

In 2016, malaria caused an estimated 216 million illnesses and 445,000 confirmed deaths globally. The disease is caused by a parasite, and mosquitos infected with the parasite transmit them to humans when they bite. In humans, the parasites enter the body and head to the liver before spending part of their life cycle in red blood cells, which cause the symptoms of the disease.

Prevention efforts have reduced the burden of malaria but eliminating the disease will require new tools. One option is to use vaccines. The world’s first malaria vaccine – a so-called pre-erythrocytic vaccine (PEV) – targets the stages preceding the parasite reaching the liver. This vaccine prevents malaria parasites from infecting people, but it is only partially effective. Scientists are also developing transmission-blocking vaccines (TBVs). These TBVs block the development of malaria parasites in mosquitos that bite vaccinated humans. So far, the most promising TBV candidates are also only partly effective.

It is possible that using PEV and TBV vaccines together could boost their effectiveness, since the TBV vaccines reduce the number of parasites that infect each mosquito. This means that fewer parasites are injected into the next person. Currently, the PEVs work better when there are fewer parasites infecting a person.

Now, Sherrard-Smith et al. show that combining TBVs with PEVs enhances their antimalarial effects. In the experiments, Sherrard-Smith et al. treated mice with either TBV or PEV vaccines, or both. Then, the mice were exposed to mosquitos infected with the malaria parasite. As expected, the TBV and PEV treatments were only partially effective when used alone. But exposing the mice to both TBVs and PEVs eliminated the parasites from the mosquitos and the mice.

The combined benefit of TBVs and PEVs were greater than would be expected if either vaccine was acting alone and the effects were simply multiplied, suggesting they enhance each other’s effects. More studies of TBVs in humans are needed to prove they are safe and effective in the real world. More studies also are needed to confirm what Sherrard-Smith et al. found in mice would happen in humans treated with a combination of TBV and PEV vaccines. But if such future studies prove this combination approach is effective, it could be a powerful tool in the fight against malaria.

Introduction

Malaria remains a major global health challenge with an estimated 216 million new cases and 445,000 deaths in 2016 (World Health Organization, 2017). Whilst current tools have substantially reduced the global burden of disease, new tools will be needed to achieve malaria elimination (Walker et al., 2016). Early development of malaria vaccines focused on either the pre-erythrocytic stage vaccine (PEV) – eliciting an immune response to prevent incoming sporozoites from establishing patent infection – or blood-stage – boosting natural responses to surface proteins on the infected erythrocytes (Schwartz et al., 2012). The first malaria vaccine RTS,S/AS01 to complete Phase III trials is a PEV vaccine and has been demonstrated to be partially effective, reducing clinical incidence in 5 – 17-month-old children by 36.3% (95%CI: 31.8 – 40.5%) over 40 months follow-up (RTSS Clinical Trials Partnership, 2015). Further candidate PEV vaccines include those that achieve protective immunity through irradiated/chemo-attenuated Plasmodium falciparum sporozoites, (e.g. PfSPZ vaccines [Seder et al., 2013]), those that use viral vectors to induce T-cell responses to provide protection (de Barra et al., 2014MVVC group et al., 2015) and the promising next-generation RTS,S-like vaccine, R21 (Collins et al., 2017). A range of vaccines that target human-to-mosquito transmission by attacking sexual, sporogonic, and/or mosquito antigens (transmission-blocking vaccines, TBV) are also under development (Talaat et al., 2016; Wu et al., 2008). Pre-clinical investigations have identified multiple antigens (e.g. Pfs25, P230, P48/45) as targets for TBV candidates that, when administered, can reduce transmission to mosquitoes (Hoffman et al., 2015; Sauerwein and Richie, 2015), but complete, or reproducible, translation to the clinic has not been achieved so far (Talaat et al., 2016; Hoffman et al., 2015; Sauerwein and Richie, 2015).

One of the major challenges encountered in developing PEV malaria vaccines is the partial protection achieved against each exposure, despite high levels of induced antibody titres. It has been hypothesized that this may be in part due to the over-dispersed distribution of sporozoites in each infectious bite, such that despite inducing a high per-parasite killing efficacy, the probability that at least one parasite reaches the liver and progresses to blood-stage infection remains high (White et al., 2013; Bejon et al., 2005). The classical approach to overcoming this is to attempt to further increase either the quantity, breadth or quality of the immune response (Remarque et al., 2012; Courtin et al., 2009; Chaudhury et al., 2016). We hypothesized that an alternative mechanism would be to combine a PEV with approaches that reduce the number of sporozoites in the mosquito salivary glands. TBVs have been demonstrated to act in this way, reducing ookinete and sporozoite density (Bompard et al., 2017; Blagborough et al., 2013). We sought therefore to identify whether this mechanism could result in synergistic interactions between PEVs and TBVs co-administered within a population.

To test this hypothesis, we used an established murine population assay to investigate the clearance of malaria over multiple generations in a controlled laboratory environment (Blagborough et al., 2013). Here, the rodent malaria parasite Plasmodium berghei is passed between populations of mice by the direct feeding of Anopheles stephensi mosquitoes. To simulate the antibody response to a PEV, a monoclonal antibody (mAb-3D11) - which targets the same corresponding parasite circumsporozoite protein (CSP) as RTS,S – was passively transferred (intravenously) into mice. To act as a partially effective PEV (broadly comparable to RTS,S), a mAb-3D11 dose was selected which reduces mosquito-to-mouse transmission probability by ~50% (as evaluated in naive mouse populations, transfused with differing doses of 3D11, challenged with five mosquito bites, see Materials and methods). Sterilizing immunity of 47.2% was titrated over multiple challenges. The complementary actions of a TBV antibody response were simulated using an anti-Pfs25 monoclonal antibody 4B7 (mAb-4B7), administered by passive transfer, which targets the same parasite stages as the most currently advanced human TBV candidate, Pfs25 (Talaat et al., 2016). This well-established transmission-blocking monoclonal antibody was used in combination with a transgenic P. berghei (PbPfs25DR3) parasite that expresses Pfs25 in place of its rodent homologue. PbPfs25DR3 is phenotypically indistinguishable to WT P. berghei, expresses Pfs25 on the surface of the zygote/ookinete, and has been used previously to assay a range of TBVs (Goodman et al., 2011; Kapulu et al., 2015). A series of transfused mAb-4B7 doses were tested in multiple (n = 6) direct feeding assays to titrate the appropriate doses to generate a 50%, 65% and 85% reduction in transmission to the mosquito (measured as reduction in oocyst prevalence) (see Materials and methods).

We undertook a series of experiments with either PEV alone, TBV alone at three different efficacies (50%, 65% and 85%), or combinations of the two across four generations of transmission. For each experiment mice were exposed to either 1, 2, 5 or 10 infectious mosquito bites to allow estimation of combined transmission-blocking efficacies between 20% and 100% (Materials and methods).

Results

At lower TBV antibody dose exposure levels (50% and 65%), the probability of eliminating all parasites from the mouse/mosquito populations was greater when PEV and TBV antibodies were administered together compared to singly, irrespective of the dose of the TBV antibody administered (Figure 1). Using statistical methods that explicitly capture parasite density and account for the impact of the interventions on both the prevalence and density of infection (Sherrard-Smith et al., 2017), we estimated PEV antibody alone to reduce the prevalence of infection by 48.0% (95% credible interval, CrI, 36.6–58.0%). Similarly, use of TBV antibody alone reduced the prevalence of infection by 33.9% (95% CrI: 18.2–47.4%), 74.3% (65.7%–82.4%) and 95.8% (90.2%–100%) for the 50%, 65% and 85% individual efficacy titres, respectively. If the actions of the two antibody types were to act independently, the predicted combined efficacy would be 83.3% (79.1–87.0%). A substantially higher efficacy of 90.8% (86.7–94.2%) (p=0.0035) was observed in the PEV +TBV antibody group, indicating a synergistic interaction (Table 1). Here, the 95% Credible Intervals did not overlap the median estimates, demonstrating a significant difference between the two treatments. The same relationship was observed when examining vaccine efficacy against parasite density (p=0.0025) (Table 1).

Figure 1. Summary outcome data.

The number in each box (and the color) shows the percentage of mice infected for each treatment arm of the experiment by transmission cycle and biting rate (the number of potentially infectious mosquito bites received per mouse). In transmission cycle 0, all mice are infected (not shown), where a TBV antibody is administered (top row: purple and blue) infections in mice are progressively reduced. The antibody works best at the higher dose (TBV 85%) and lower biting rates. The PEV antibody (lower row: yellow and green) is effective at lower biting rates (where each mouse received one or two potentially infectious mosquito bites per transmission cycle) but is not able to reduce infection at higher biting rates. In combination, at any biting rate, the combined antibodies (lower row: orange) always cleared infections by transmission cycle 2.

Figure 1.

Figure 1—figure supplement 1. Adapted from Malaria Journal (Sherrard-Smith et al., 2017) A graphical outline of the multi-generational transmission experiment (A) and its mathematical representation (B).

Figure 1—figure supplement 1.

(A) The mosquito-mouse model system. Five female (TO) mice (6–8 weeks old, Harlan, UK) were treated with phenylhydrazine, and, 3 days later, were infected with 106 P. berghei PbPfs25DR3 (Goodman et al., 2011). Three days later, groups of infected mice were treated with the TBV antibody. After 1 hr, the mice were anaesthetised and 500 An. stephensi mosquitoes (line SD 500, starved for 24 hr) fed randomly on the five infected mice within each group. Mosquitoes were maintained as described in (Blagborough et al., 2013). After 10 days, a sub-sample of 50 mosquitoes were microscopically examined to measure oocyst intensity and prevalence. After 21 days post-feeding, sporozoites are present in the salivary glands and are maximally infectious to the vertebrate host (Blagborough et al., 2013). At this point, pre-defined numbers of mosquitoes (to simulate mosquito biting rates of 1, 2, 5 and 10 mosquito bites per mouse) were then randomly selected from the remaining mosquitoes and fed, for 20 min, on anesthetized mice from a naive cohort. Each group of mice (five mice per group) either received the PEV antibody or no -intervention (negative control). Engorged mosquitoes were microscopically examined immediately after feeding to determine the number of sporozoites in the salivary glands. After 10 days, blood smears from each mouse were microscopically examined to determine the percentage parasitemia. These five mice were then given either the TBV antibody at the desired dose to achieve a 50%, 65% or 85% reduction in oocyst prevalence as required, or no intervention/control (in accordance with the respective treatment arm). A new cohort of 500 naive mosquitoes was then allowed to blood feed on the mice. This mouse-to-mouse transmission cycle was repeated to a maximum of four cycles after the seeding mouse population or until no parasites had been detected in the system for two successive transmission cycles. (B) The statistical model mirrored the experimental set up. The initial parasite density generated by injecting mice N0, the oocyst intensity O’ and the parasite density in mice transmitted by mosquito bites N, are modelled assuming zero-inflated negative binomial distributions. The sporozoite count S data for the biting mosquitoes were censored which means that the data are modelled as a multinomial distribution. These distributions are defined by the mean (µ, o, s for parasite density in mice, oocyst counts and sporozoite counts in mosquitoes) and dispersion (φ, τ, σ for parasite density in mice, oocyst counts and sporozoite counts in mosquitoes) and zero-inflation (πP, πV) parameters. Parameters from the previous life stage are used to inform the next (the respective parameter informing the subsequent life-stage is indicated by the arrows). The biting effect m is modelled when sporozoites in mosquitoes propagate parasite infections in mice for each transmission cycle i and treatment arm t. All care and handling of animals strictly followed the Guidelines for Animal Care and Use prepared by Imperial College London and was performed under the UK Home Office Licence 70/7185. Supplementary information Table 1—source data 1 (separate excel file). Data file of the raw data for parasite densities in mice and mosquitoes.
Open in a new tab

Table 1. Summary of the density model estimation of efficacy against prevalence and parasite density for the transmission blocking (TBV) and pre-erythrocytic (PEV) antibodies that were administered either alone or together to reduce malaria parasites in mice.

The interaction between the two antibodies are measured using the ratio of observed estimates for combination treatments compared to the expected efficacy were vaccine antibodies acting independently using the simulated posterior draws from the density model (Sherrard-Smith et al., 2017). A value of less than one indicates an antagonistic interaction, = 1 suggests antibodies are acting independently, and greater than one shows synergy.

Table 1—source data 1. The raw data used for analysis.
elife-35213-table1-data1.xlsx (112.7KB, xlsx)
DOI: 10.7554/eLife.35213.006
Intervention arm Efficacy Synergy
Reduction in prevalence (95% credible intervals) Reduction in density (95% credible intervals) Prevalence p-value Density p-value
Individual vaccine efficacies
 All TBV combined 68.0 (61.1–74.1) 51.5 (6.8–72.9)
 TBV: MAb-4B7 (50%) 33.9 (18.2–47.4) 13.6 (0–47.5)
 TBV: MAb-4B7 (65%) 74.3 (65.7–82.4) 69.3 (47.8–84.8)
 TBV: MAb-4B7 (85%) 95.8 (90.2–100) 94.2 (79.1–100)
 PEV: Mab-3D11 (50%) 48.0 (36.6–58.0) 2.8 (0–25.2)
Combined vaccine efficacies
 PEV and All TBV combined 90.8 (86.9–94.2) 90.9 (79.0–96.4) 1.09 (1.02–1.18) p<0.0035 2.08 (1.20–5.02) p<0.0025
 PEV (50%) and MAb-4B7 (50%) 82.2 (74.6–88.9) 85.8 (75.6–92.8) 1.27 (1.07–1.60) p<0.0015 19.04 (1.56–75.16) p<0.0001
 PEV (50%) and MAb-4B7 (65%) 92.8 (86.1 - 98.6) 93.2 (75.4 - 99.7) 1.07 (0.98 - 1.17) p<0.0675 1.36 (1.02 - 1.97) p<0.02
 PEV (50%) and MAb-4B7 (85%) 96.9 (91.2 – 100) 94.8 (74.4 - 100) 0.99 (0.93 - 1.04) p<0.5435 1.01 (0.78 - 1.22) p<0.3755
Open in a new tab

Sub-dividing the data by TBV antibody dose, the greatest synergistic enhancement in efficacy against parasite prevalence was seen at lower doses of functional TBV antibodies (Figure 2). A TBV antibody dose which reduces mouse-to-mosquito transmission by 50% increased the efficacy of PEV antibody prevalence to 82.2% (74.6–88.9%) compared to an expected 65% (57.7–73.2%) efficacy if the vaccines acted independently, a strong indication of synergy (p=0.0015). Similar synergistic effects against parasite density were observed (Figure 2, p <0.0001). Weaker synergistic effects were observed against parasite prevalence and density for the PEV +TBV antibody at the 65% dose (Figure 2, p=0.0675, 0.02, respectively) (Table 1). At the highest TBV antibody dose (85%), the TBV alone already reduced parasites in the population to low levels, hence there was insufficient power to detect further synergy between the interventions as all parasites were eliminated from the experimental population (Figure 1).

Figure 2. The efficacy of vaccine antibody combinations against parasite prevalence (the proportion of infected hosts) (A) and density (the mean parasite density per host, measured as the number of infected red blood cells out of a total subsample of 1200 erythrocytes) (B) in mice.

Figure 2.

Open in a new tab

The observed efficacy of PEV monoclonal antibody mAb-3D11 at a dose previously shown to reduce transmission to mice by ~50% when exposed to five infectious mosquito bites. The efficacy of the TBV mAb-4B7 at doses previously shown to reduce transmission to mosquitoes by 50%, 65% and 85% (blue section, purple lines). The efficacy of antibodies administered together (gold sections) that were observed (gold) or expected (red) were efficacies for each antibody acting independently (mean (point) and 95% credible intervals (lines) shown). Asterisks indicate increasing levels of support of synergy (p<0.1, p<0.05*, p<0.01**, p<0.001***).

The impact of circulating TBV antibody on the reduction of parasites within the mosquito explains the greater efficacy of the PEV antibody in the combination treatment groups. The presence of TBV antibody (mAb-4B7) reduced oocyst counts in infected mosquitoes (ANOVA: F1,1525 = 75.3, p<0.0001). Similarly, TBV antibody presence reduced sporozoite density in infected mosquitoes (ANOVA: F1,707 = 163.9, p<0.0001). Figure 3A,B and C further illustrate the effect that TBVs have on sporozoite density distribution for the TBV-50%, 65% and 85% single treatment groups respectively. At each dose, the tail of the distribution of sporozoites is curtailed progressively across transmission cycles. Figure 3D illustrates that the efficacy of the PEV is density-dependent, with higher efficacy achieved when mosquitoes have lower sporozoite density.

Figure 3. The impact of TBV monoclonal antibody mAb-4b7 on PEV mAb-3D11 efficacy.

Figure 3.

Open in a new tab

The TBV antibody alone reduces the tail of the sporozoite distribution in mosquitoes across transmission cycles for the (A) 50% dose, (B) 65% dose and (C) 85% dose. (A–C) demonstrate that the sporozoite scores (measured on a log scale; 0 indicates no sporozoites; 1 = 1–10 sporozoites; 2 = 11–100 sporozoites; 3 = 101–1000 sporozoite and; 4 =>1000 sporozoites per mosquito) tend toward zero for successive transmission rounds. (D) The efficacy of the PEV antibodies to prevent mosquito-to-mouse-to-mosquito transmission (a percentage reduction in sporozoite infections in mosquitoes) is greatest at lower mosquito parasite densities (as assessed by sporozoite score following blood-feeding).

Discussion

The efficacy of multiple PEV and TBV candidates against rodent and human parasites have been shown to depend on parasite density; TBV (anti-Pfs25, anti-Pfs48/45 and immune blocking serum) efficacy decreases with increased parasite dose (Churcher et al., 2012; Miura et al., 2016) and a representative PEV (RTS,S) only provides sterilizing immunity in volunteers against lightly infected mosquitoes (Churcher et al., 2017). This suggests that both types of vaccine can halt transmission against a defined (but currently uncharacterized) quantity of parasites, which is enough to prevent onward infection in lightly infected mosquitoes/humans, but that onward transmission is still possible from heavily infected mosquitoes or individuals.

Here, a partially effective TBV antibody reduced the number of parasites in infected mosquitoes, ensuring that the PEV antibodies encounter fewer parasites than would otherwise be expected if only a single antibody/vaccine class was administered in isolation. Thus, the subsequently reduced parasite burden increased the efficacy of the PEV when co-administered with a TBV. Potentially, a synergistic response could be induced by an unspecified biochemical or immunological interaction between the two vaccines. This explanation can be discounted within this system as the experimental design results in mosquito-to-mouse transmission being measured prior to the administration of a transmission-blocking intervention (passive transfer of mAb-4B7 1 hr prior to blood feed) as a new, naive batch of mice were infected in each generation.

The greatest synergy was observed in the lower TBV dose group, although it is likely to operate across all TBV and PEV doses when vaccine reduces parasite density but fails to clear infection from host or vector. The 85% TBV dose administered alone eliminated the parasite over a single generation without the action of the PEV so there was no opportunity to show synergy. A 100% efficacious PEV or TBV would not require augmenting with an alternative vaccine, although their efficacy is still likely to drop over time as antibodies decay so combining highly effective vaccine may still be advantageous depending on the relative rates of antibody loss.

While the direct translatability of rodent experiments to human health is variable, this approach is invaluable to demonstrate unequivocally that the mechanism behind the observed synergy is the direct result of TBV antibody reducing parasite density in infected mice and thereby enabling the density-dependent PEV antibody to be optimal (Figure 3). This mechanism is very likely to mirror that for humans, which cannot be tested directly due to ethical considerations and complex environmental variation. Whilst the murine system uses P. berghei, the mechanism of action of the PEV antibodies administered is matched to the antibody-based mechanism of the RTS,S vaccine; that is sporozoite invasion of the liver is inhibited by the presence of CSP-targeted antibodies in mice both in vivo and ex vivo (Grüner et al., 2003). The P. berghei strain used here is genetically modified to express the human TBV candidate, P. falciparum P25 (Pfs25) in place of its P. berghei counterpart. Thus, a proven anti-falciparum TBV mAb (4B7) can be used directly within the model (Goodman et al., 2011). The evidence that co-administering TBV and PEV antibodies can accelerate toward controlling malaria transmission is a first step toward trialing such combinations in more natural parasite-vector-host combinations and environments. There is good reason to believe that the population dynamics of parasites and partially effective vaccines may be similar in human malaria. Transmission of human malaria from human-to-mosquito and mosquito-to-human is also considered to depend on the density of the parasite (Churcher et al., 2013; Sinden et al., 2007). The average number of oocysts in wild caught mosquitoes is likely to be substantially lower than the numbers observed in the rodent system (Rosenberg, 2008) but oocyst distribution is highly over-dispersed (Medley et al., 1993) meaning that some mosquitoes have very-high-density infections. These highly infected mosquitoes are likely to be more infectious, so reducing their frequency through adding a TBV, could have additional impact on overall transmission. The epidemiological importance of any synergistic interaction between vaccine types in the field is hard to predict and will depend on many confounding factors such as human immunity, drug treatment, vector susceptibility, antigen escape, amongst others. Transmission is likely to be highly heterogeneous, caused by factors such as vaccine non-responders and super-transmitting hosts. The impact of different types of heterogeneity can be investigated under controlled laboratory scenarios using the murine population assay, varying the vaccinated coverage, antibody dose and changing biting heterogeneity within a population. This could help understand the relative importance of these different heterogeneities and could be used to support the design of appropriately powered Phase III trials (or alternative trial designs) to fully assess the impact of combining vaccine components with alternative mechanisms of action.

There is no ‘magic bullet’ intervention against malaria and the current global strategy is to combine vector control and drug treatment tools in a timely manner to move towards malaria elimination. Our results suggest that the same approach might be taken for the use of vaccines and comprises the first practical demonstration that combining TBVs and PEVs may have auxiliary benefits. Synergism between PEV and TBVs could potentially enhance the efficacy of the current PEV vaccines, resulting in reduced burden and potentially elimination in areas where it was not previously possible. The development of novel anti-malarial vaccines is both costly and time-consuming. Combining partially effective vaccines of differing anti-parasitic classes may be therefore a pragmatic and powerful way to accelerate malaria elimination efforts. Synergism between PEV, TBVs and potentially a blood-stage vaccine (either administered separately or as a multi-component vaccine) could potentially enhance the efficacy of single vaccines, resulting in reduced burden and potentially elimination in areas where it was not previously possible.

Materials and methods

Key resources table.

Resource type (species) or resource Designation Reference Identifiers
Antibody mAb-4b7 (Stura et al., 1994) RRID:AB_2728658
Antibody mAb-3D11 (Mishra et al., 2012) RRID:AB_2728657
Open in a new tab

Transmission-blocking vaccine surrogate: monoclonal antibody 4B7 (mAb-4B7)

The TBV mAb-4B7 neutralises the protein Pfs25 in sexual stages of the human malaria P. falciparum and reduces transmission of the parasite from host-to-mosquito (Stura et al., 1994). The transgenic murine malaria parasite, P. berghei PbPfs25DR3, expressing native Pfs25 in place of its rodent homologue, was used so that the same TBV antibody candidate could be examined within a mouse model (Goodman et al., 2011). MAb-4B7 was administered and examined at sub-optimal concentrations titrated to reduce oocyst prevalence in the mosquito midgut (as assessed using a direct feeding assay) by either 50, 65 or 85%. Given the severity of malaria, the WHO, the Strategic Advisory Group of Experts (SAGE) on Immunization and the Malaria Policy Advisory Committee (MPAC) recommended the RTS,S vaccine could be implemented in pilot countries in October 2015 (http://www.malariavaccine.org/malaria-and-vaccines/first-generation-vaccine/rtss, accessed 04/04/2018) when the vaccine was demonstrating relatively low efficacies of just 36.3% in children aged 5 to 17 months (RTSS Clinical Trials Partnership, 2015). These TBV doses were chosen to bridge a range of malaria vaccine efficacies that might be acceptable by WHO, SAGE and MPAC. Briefly, to titrate the appropriate dose, female Tuck Ordinary (TO) mice (6–8 weeks old, Harlan, UK) were treated with phenylhydrazine, and three days later, infected with 106 P. berghei PbPfs25DR3 (Goodman et al., 2011). Three days later, infected mice were injected intravenously (i.v.) with 200 µl of purified mAb-4B7 at a range of doses. Negative control mice were transfused with 200 µl of phosphate buffered saline (PBS). After 1 hr, mice were anesthetised and 50 Anopheles stephensi mosquitoes (line SD 500, previously starved for 24 hr) were allowed to feed on each individual mouse. Mosquitoes were maintained as described in (Blagborough et al., 2013), and after 10 days, 50 mosquitoes were dissected and microscopically examined to measure oocyst intensity and prevalence. This was repeated five times, with i.v. administered doses of mAb-4B7 ranging from 0 µg to 750 µg. Prevalence efficacy was estimated as a function of mAb-4B7 concentration using a generalised linear model framework (Bolker et al., 2009) in which experimental replicate was treated as a random effect. A Gompertz function (Churcher et al., 2013) was fitted to the data using maximum likelihood methods. Mean concentrations were estimated using the best-fitting model (determined by log-likelihood tests) with 95% confidence intervals obtained from the profile likelihood. We estimated that a mAb-4B7 dose of 284.2 µg i.v (244.7–337.3 µg) was required to achieve a reduction in prevalence of 50%, a dose of 371.8 µg i.v (319.8–442.8 µg) for 65% reduction and a dose of 629.5 µg i.v (525–777.1 µg) for an 85% reduction. These calculated doses were then used in the mosquito-mouse model system as described below.

Pre-erythrocytic vaccine surrogate: monoclonal antibody 3D11 (mAb-3D11)

The anti-P. berghei CSP mAb-3D11 (Mishra et al., 2012) is mechanistically similar to the recently registered RTS,S vaccine for human malaria, in that the presence of CSP-targeted antibodies in mice inhibit sporozoite invasion of the liver both in vivo and ex vivo (Grüner et al., 2003). An appropriate dose for mAb-3D11 was estimated from 40 individual passive transfers, administering a range of mAb-3D11 doses (0–150 µg i.v.) to mice (5 to 10 mice per experiment) and determining the prevalence efficacy at the given dose. A logistic function was fitted to these data using RStan (Stan Development Team, 2017) to determine the mean dose and 95% credible intervals that produces a ~50% reduction in the probability of infection. Consequently, mAb-3D11 antibody was administered at a single sub-optimal dose (50 µg i.v.) that prevented 47.2% (38.0–62.0% 95%CI) of transmission to mice that each received 5 potentially infectious mosquito bites. This dose was selected to match the approximate observed protection by RTS,S in human clinical trials.

The mosquito-mouse model system

The mouse-to-mouse transmission model has been described in detail previously (Upton et al., 2015; Blagborough et al., 2013) (Figure 1—figure supplement 1). Briefly, five female (TO) mice (6–8 weeks old, Harlan, UK) were treated with phenylhydrazine, and, 3 days later, were infected with 106 P. berghei PbPfs25DR3 (Goodman et al., 2011). Three days later, groups of infected mice were treated with the TBV antibody. After 1 hr, the mice were anesthetised and 500 An. stephensi mosquitoes (line SD 500, starved for 24 hr) fed randomly on the five infected mice within each group. Mosquitoes were maintained as described in Blagborough et al., 2013. After 10 days, a sub-sample of 50 mosquitoes were microscopically examined to measure oocyst intensity and prevalence. After 21 days post-feeding, sporozoites are present in the salivary glands and are maximally infectious to the vertebrate host (Blagborough et al., 2013). At this point, pre-defined numbers of mosquitoes (to simulate mosquito biting rates of 1, 2, 5 and 10 mosquito bites per mouse) were then randomly selected from the remaining mosquitoes and fed, for 20 min, on anesthetized mice from a naïve cohort. The mosquito biting rate is an aspect of the experimental design that can be varied to be able to estimate the effect size more precisely. If the mosquito biting rate is small (say 1 or 2), the probability that the infection is eliminated rapidly in the intervention arm of the experiment is high (>80%) for TBD/TBV with efficacies above 40%. Thus, we cannot discriminate at a low mosquito biting rate between a TBD/TBV with 60% efficacy and one with 80% efficacy (they both eliminate). However, we do obtain a high degree of discrimination between an efficacy of 20% and one of 40%. Thus, a small mosquito biting rate is needed to get a precise estimate of the effect size of a TBD/TBV with lower efficacy. The converse also holds, so that a high mosquito biting rate (up to around 10 based on our initial experiment) is needed to obtain a precise estimate of a TBV/TBD with >80% efficacy. Using multiple mosquito biting rates increases the overall precision of our estimate of prevalence efficacy.

Each group of mice (five mice per group) either received the PEV antibody or no -intervention (negative control). Engorged mosquitoes were microscopically examined immediately after feeding to determine the number of sporozoites in the salivary glands. After 10 days, blood smears from each mouse were microscopically examined to determine the percentage parasitemia. These five mice were then given either the TBV antibody at the desired dose to achieve a 50%, 65% or 85% reduction in oocyst prevalence as required, or no intervention/control (in accordance with the respective treatment arm). A new cohort of 500 naive mosquitoes was then allowed to blood feed on the mice. This mouse-to-mouse transmission cycle was repeated to a maximum of four cycles after the seeding mouse population or until no parasites had been detected in the system for two successive transmission cycles. The PEV and TBV antibodies at each dose (corresponding to a reduction in transmission to mosquitoes of 50%, 65% and 85%) were tested singly and in combination.

Initial parasite density was measured by counting the number of infected red blood cells (out of a total subsample of 1200 erythrocytes). The number of sporozoites in the salivary glands following blood feeding was counted on the logarithmic scale (scores of 0–4 representing 0, 1–10, 11–100, 101–1000, 1000 + sporozoites, respectively). The data are provided in Table 1—source data 1.

Ethics statement

All animal procedures were performed in accordance with the terms of the UK Animals (Scientific Procedures) Act (PPL 70/8788) and were approved by the Imperial College Animal Welfare and Ethical Review Body (AWERB) LASA guidelines were adhered to at all points. The Office of Laboratory Animal Welfare Assurance for Imperial College covers all Public Health Service supported activities involving live vertebrates in the US (no. A5634-01).

Statistical analysis

The complexity of the population assay requires non-standard methods of statistical analyses that can account for the non-linear dynamics of transmission and stochastic fluctuations seen by the relatively small number of mice used in each generation and treatment arm. These methods need to be able to determine whether the interaction between the different antibodies, that simulate vaccine-triggered antibodies, is below what would be expected if vaccine effects were less strong than expected if effects were multiplied (sub-multiplicative), independent of the presence of the other vaccine (multiplicative) or synergistic, in that effects are enhanced for one or both vaccine types (super-multiplicative).

A density model was developed specifically for this purpose (described in full, [Sherrard-Smith et al., 2017], Figure 1—figure supplement 1). The structure of the model captures the experimental set up and fits explicitly to parasite densities during successive life stages to generate more precise estimates of simulated vaccine efficacy than the direct comparison of raw data alone, which can fluctuate widely due to chance (as each generation only has five mice) (Table 1—source data 1). Stochastic elimination (or resurgence) is possible in the mouse system given the ethical necessity to keep the mouse populations in each generation small; as only five mice are used so transmission could be halted or enhanced by natural variability in the physiological response from each individual mouse. The statistical mode, however, explicitly addresses this variation by modeling the distribution of pathogens at each stage of transmission for each mouse individually. By explicitly incorporating the heterogeneity in the mouse pathogen load the model avoids bias in the inference of the transmission process itself. All parameters were fitted jointly using a Bayesian posterior distribution in RStan (version 2.13.1, [Stan Development Team, 2017]). To ensure robust fits, a non-centered parameterization method was employed (Papaspiliopoulos et al., 2007; Betancourt and Girolami, 2015). The model parameter fitting was achieved using a Hamiltonian Monte Carlo method (Stan Development Team, 2017), warmup was 500 and the subsequent 500 samples from each chain (n = 4) were used for the posterior predictive checks (Sherrard-Smith et al., 2017). The model was validated by visualizing the observed raw data measurements of parasite density in mice, the oocyst counts and the logarithmic counts of sporozoites in mosquitoes against model predictions. The data were analyzed at different scales, first taking all data together before breaking down the impact by the dose of the TBV antibody.

The prevalence efficacy against infections in mice is the percentage difference in the proportion of infected hosts between the control and treatment arms of the experiment. The parasite density efficacy against infections in mice is the percentage difference in the mean parasite density per host between the control and treatment arms of the experiment. (Similarly, efficacies can be calculated for the reduction in oocysts or sporozoites in mosquito populations.)

Efficacy estimates were generated for each arm of the experiment, for each posterior draw of the model (2000 posterior draws). This allows mean and 95% credible intervals to be calculated for each treatment group (c) and across mosquito biting rates (m) and transmission cycles (i). Let Pc,m,ijindicate the prevalence of infected mice (j = 1) or the mean asexual parasite density in the mouse population (j = 2). Treatment arm 0 represents the control data, and c indicates treatments 1 to 7 (TBV antibody at 50%, 65%, 85% dose singly, PEV antibody singly, PEV and TBV antibody at 50%, 65% and 85% dose together), such that,

Ec,m,ij=P0,m,ijPc,m,ijP0,m,ij×100 (1)

where Ec,m,ij is either the parasite prevalence efficacy (j = 1) or density efficacy (j = 2) against infections in mice as estimated by the posterior predictions of the density model (Table 1).

To statistically assess whether the interaction between PEV and TBV antibodies are antagonistic, independent or synergistic, efficacy estimates against infections in mice for combined antibody treatments were compared to the expected estimates if antibodies had an independent impact (expected efficacy). To estimate this expected efficacy the single antibody treatment groups were combined, as follows (VanderWeele and Knol, 2014):

ExpectedEfficacy=Epev*(1Etbv,d)+Etbv,d (2)

where Etbv,d is the prevalence or density efficacy for the TBV antibody treatment alone (at the specified TBV dose of d = 50%, 65% or 85%), and Epev is the prevalence or density efficacy for the PEV alone. The ratio between efficacies for the combined treatments and the expected efficacy for matched treatments was used to assess synergy. A synergistic interaction is indicated when this ratio is greater than 1, an independent interaction when equal to one and an antagonistic impact if less than 1 (Figure 4). The 95% credible intervals were calculated to give statistical support. Statistical evidence of a difference in treatment and control experiments (p-value) was defined as one minus the proportion of iterations from the model simulations that were greater than 1.

Figure 4. Evidence of a synergistic effect of parasite prevalence (A–D) or parasite density (E–H) of combining TBV monoclonal antibody (mAb-4B7) with PEV mAb-3D11.

Figure 4.

Open in a new tab

The frequency histograms show the probability that antibodies administered together have a higher efficacy than if they acted independently. In all panels, the vertical black line highlights the value 1, above this line indicates synergy, below it denotes an antagonistic interaction and falling at one indicates that the antibodies are acting independently (evidence for synergy p<0.1., p<0.05*, p<0.01**, p<0.001***). Taking all data together (A and E), there is a synergistic effect of combining vaccine antibodies as the majority of iterations fall above 1. This effect is stronger at lower doses of mAb-4B7 (B, C, F and G, note the different x-axes values indicating stronger support for lower TBV antibody doses), and stronger against parasite density (E–H) than parasite prevalence.

The observed synergy can be explained because the presence of TBV antibody reduces the sporozoite score (as a measure of parasite density in the mosquito population) which allows the PEV antibodies to achieve a greater efficiency. To understand whether the combined TBV antibody treatments improved the action of the PEV at higher parasite densities, the raw data recording the sporozoite scores of each mouse in the single treatment TBV antibody groups were plotted for each dose and across transmission cycles to demonstrate that there are progressively more mosquitoes without infection and progressively fewer mosquitoes with heavy infections (Figure 3). This highlights that the PEV in the combined treatment groups is acting against progressively fewer parasites in each transmission cycle because of the initial action of the TBV antibody. Simple analysis of variance was performed to confirm that the presence of the respective antibody type (PEV acting against infections in mice, TBV acting against sporozoites in mosquitoes), as a binary covariate, could explain reduced parasite counts in mosquitoes or mice. To demonstrate that the PEV antibody has a density-dependent impact, binomial logistic regression curves were fitted to determine the relationship between the prevalence efficacy of the PEV antibody and the parasite density in mosquitoes (measured as mean sporozoite score for each mosquito biting rate and transmission cycle, n = 16). Parameters describing the regression curves were fitted using a Bayesian posterior distribution in RStan (version 2.13.1, [Stan Development Team, 2017]). The model parameter fitting was achieved using a Hamiltonian Monte Carlo method (Stan Development Team, 2017), warmup was 1000 and the subsequent 1000 samples from each chain (n = 4) were used for the posterior predictive checks (Stan Development Team, 2017). All data analysis were conducted using the statistical software R (version 3.2.2; [Core Team, 2014]).

Acknowledgements

The data used in this manuscript are listed in Supplementary information Table 1—source data 1. We thank Mark Tunnicliff for mosquito production. AMB, TSC, AG, ESS and MJM formulated the theory and prediction for the concepts presented. AMB, TSC and KAS contributed to experimental conception and design. Acquisition, analysis and/or interpretation of data were completed by ESS, MB, AMB, KAS, LMU and FA. ESS, TSC, AG and AMB drafted the article and all authors revised it critically for important intellectual content. The authors acknowledge PATH’s Malaria Vaccine Initiative for funding this work. TSC thank the UK Medical Research Council (MRC)/UK Department for International Development (DFID) under the MRC/DFID Concordat agreement. AMB thanks the MRC (grant number MR/N00227X/1) for funding. MB is supported under EPSRC grant EP/J016934/1.

Funding Statement

The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication.

Contributor Information

Ellie Sherrard-Smith, Email: e.sherrard-smith@imperial.ac.uk.

Urszula Krzych, Walter Reed Army Institute of Research, United States.

Funding Information

This paper was supported by the following grants:

  • PATH GAT.0888-11-06546-COL to Azra C Ghani, Thomas S Churcher, Andrew M Blagborough.

  • Medical Research Council MR/N00227X/1 to Andrew M Blagborough.

  • Engineering and Physical Sciences Research Council EP/J016934/1 to Michael Betancourt.

Additional information

Competing interests

No competing interests declared.

Author contributions

Formal analysis, Validation, Investigation, Visualization, Methodology, Writing—original draft, Writing—review and editing.

Data curation, Investigation, Methodology, Writing—review and editing.

Formal analysis, Validation, Methodology, Writing—review and editing.

Data curation, Methodology, Writing—review and editing.

Data curation, Methodology, Writing—review and editing.

Conceptualization, Supervision, Project administration, Writing—review and editing.

Conceptualization, Supervision, Funding acquisition, Methodology, Writing—original draft, Project administration, Writing—review and editing.

Conceptualization, Supervision, Funding acquisition, Methodology, Writing—original draft, Project administration, Writing—review and editing.

Conceptualization, Data curation, Supervision, Funding acquisition, Methodology, Writing—original draft, Writing—review and editing.

Ethics

Animal experimentation: All animal procedures were performed in accordance with the terms of the UK Animals (Scientific Procedures) Act (PPL 70/8788) and were approved by the Imperial College Animal Welfare and Ethical Review Body (AWERB) LASA guidelines were adhered to at all points. The Office of Laboratory Animal Welfare Assurance for Imperial College covers all Public Health Service supported activities involving live vertebrates in the US (no. A5634-01).

Additional files

Transparent reporting form
elife-35213-transrepform.pdf (883.7KB, pdf)
DOI: 10.7554/eLife.35213.010

Data availability

All data generated or analysed during this study are included in the manuscript and supporting files.

References

  1. Bejon P, Andrews L, Andersen RF, Dunachie S, Webster D, Walther M, Gilbert SC, Peto T, Hill AV. Calculation of liver-to-blood inocula, parasite growth rates, and preerythrocytic vaccine efficacy, from serial quantitative polymerase chain reaction studies of volunteers challenged with malaria sporozoites. The Journal of Infectious Diseases. 2005;191:619–626. doi: 10.1086/427243. [DOI] [PubMed] [Google Scholar]
  2. Betancourt M. Girolami M. Hamiltonian Monte Carlo for Hierarchical Models.”. In: Upadhyay S. K, editor; Singh U, editor; Dey D. K, editor; Logananthan A, editor. Current Trends in Bayesian Methodology with Applications. first. Boca Raton London New York: Chapman and Hall CRC Press Taylor & Francis Group; 2015. pp. 79–102. [DOI] [Google Scholar]
  3. Blagborough AM, Churcher TS, Upton LM, Ghani AC, Gething PW, Sinden RE. Transmission-blocking interventions eliminate malaria from laboratory populations. Nature Communications. 2013;4:1812. doi: 10.1038/ncomms2840. [DOI] [PMC free article] [PubMed] [Google Scholar]
  4. Bolker BM, Brooks ME, Clark CJ, Geange SW, Poulsen JR, Stevens MH, White JS. Generalized linear mixed models: a practical guide for ecology and evolution. Trends in Ecology & Evolution. 2009;24:127–135. doi: 10.1016/j.tree.2008.10.008. [DOI] [PubMed] [Google Scholar]
  5. Bompard A, Da DF, Yerbanga RS, Biswas S, Kapulu M, Bousema T, Lefèvre T, Cohuet A, Churcher TS. Evaluation of two lead malaria transmission blocking vaccine candidate antibodies in natural parasite-vector combinations. Scientific Reports. 2017;7:6766. doi: 10.1038/s41598-017-06130-1. [DOI] [PMC free article] [PubMed] [Google Scholar]
  6. Chaudhury S, Ockenhouse CF, Regules JA, Dutta S, Wallqvist A, Jongert E, Waters NC, Lemiale F, Bergmann-Leitner E. The biological function of antibodies induced by the RTS,S/AS01 malaria vaccine candidate is determined by their fine specificity. Malaria Journal. 2016;15:301. doi: 10.1186/s12936-016-1348-9. [DOI] [PMC free article] [PubMed] [Google Scholar]
  7. Churcher TS, Blagborough AM, Delves M, Ramakrishnan C, Kapulu MC, Williams AR, Biswas S, Da DF, Cohuet A, Sinden RE. Measuring the blockade of malaria transmission--an analysis of the standard membrane feeding assay. International Journal for Parasitology. 2012;42:1037–1044. doi: 10.1016/j.ijpara.2012.09.002. [DOI] [PubMed] [Google Scholar]
  8. Churcher TS, Bousema T, Walker M, Drakeley C, Schneider P, Ouédraogo AL, Basáñez MG. Predicting mosquito infection from Plasmodium falciparum gametocyte density and estimating the reservoir of infection. eLife. 2013;2:e00626. doi: 10.7554/eLife.00626. [DOI] [PMC free article] [PubMed] [Google Scholar]
  9. Churcher TS, Sinden RE, Edwards NJ, Poulton ID, Rampling TW, Brock PM, Griffin JT, Upton LM, Zakutansky SE, Sala KA, Angrisano F, Hill AV, Blagborough AM. Probability of transmission of malaria from mosquito to human is regulated by mosquito parasite density in naïve and vaccinated hosts. PLoS Pathogens. 2017;13:e1006108. doi: 10.1371/journal.ppat.1006108. [DOI] [PMC free article] [PubMed] [Google Scholar]
  10. Collins KA, Snaith R, Cottingham MG, Gilbert SC, Hill AVS. Enhancing protective immunity to malaria with a highly immunogenic virus-like particle vaccine. Scientific Reports. 2017;7:46621. doi: 10.1038/srep46621. [DOI] [PMC free article] [PubMed] [Google Scholar]
  11. Core Team R. Vienna, Austria: R Foundation for Statistical Computing; 2014. http://www.r-project.org/ [Google Scholar]
  12. Courtin D, Oesterholt M, Huismans H, Kusi K, Milet J, Badaut C, Gaye O, Roeffen W, Remarque EJ, Sauerwein R, Garcia A, Luty AJ. The quantity and quality of African children's IgG responses to merozoite surface antigens reflect protection against Plasmodium falciparum malaria. PLoS One. 2009;4:e7590. doi: 10.1371/journal.pone.0007590. [DOI] [PMC free article] [PubMed] [Google Scholar]
  13. de Barra E, Hodgson SH, Ewer KJ, Bliss CM, Hennigan K, Collins A, Berrie E, Lawrie AM, Gilbert SC, Nicosia A, McConkey SJ, Hill AV. A phase Ia study to assess the safety and immunogenicity of new malaria vaccine candidates ChAd63 CS administered alone and with MVA CS. PLoS One. 2014;9:e115161. doi: 10.1371/journal.pone.0115161. [DOI] [PMC free article] [PubMed] [Google Scholar]
  14. Goodman AL, Blagborough AM, Biswas S, Wu Y, Hill AV, Sinden RE, Draper SJ. A viral vectored prime-boost immunization regime targeting the malaria Pfs25 antigen induces transmission-blocking activity. PLoS ONE. 2011;6:e29428. doi: 10.1371/journal.pone.0029428. [DOI] [PMC free article] [PubMed] [Google Scholar]
  15. Grüner AC, Snounou G, Brahimi K, Letourneur F, Rénia L, Druilhe P. Pre-erythrocytic antigens of plasmodium falciparum: from rags to riches? Trends in Parasitology. 2003;19:74–78. doi: 10.1016/S1471-4922(02)00067-3. [DOI] [PubMed] [Google Scholar]
  16. Hoffman SL, Vekemans J, Richie TL, Duffy PE. The march toward malaria vaccines. Vaccine. 2015;33:D13–D23. doi: 10.1016/j.vaccine.2015.07.091. [DOI] [PMC free article] [PubMed] [Google Scholar]
  17. Kapulu MC, Da DF, Miura K, Li Y, Blagborough AM, Churcher TS, Nikolaeva D, Williams AR, Goodman AL, Sangare I, Turner AV, Cottingham MG, Nicosia A, Straschil U, Tsuboi T, Gilbert SC, Long CA, Sinden RE, Draper SJ, Hill AV, Cohuet A, Biswas S. Comparative assessment of transmission-blocking vaccine candidates against plasmodium falciparum. Scientific Reports. 2015;5:11193. doi: 10.1038/srep11193. [DOI] [PMC free article] [PubMed] [Google Scholar]
  18. Medley GF, Sinden RE, Fleck S, Billingsley PF, Tirawanchai N, Rodriguez MH. Heterogeneity in patterns of malarial oocyst infections in the mosquito vector. Parasitology. 1993;106:441. doi: 10.1017/S0031182000076721. [DOI] [PubMed] [Google Scholar]
  19. Mishra S, Nussenzweig RS, Nussenzweig V. Antibodies to Plasmodium circumsporozoite protein (CSP) inhibit sporozoite's cell traversal activity. Journal of Immunological Methods. 2012;377:47–52. doi: 10.1016/j.jim.2012.01.009. [DOI] [PMC free article] [PubMed] [Google Scholar]
  20. Miura K, Stone WJ, Koolen KM, Deng B, Zhou L, van Gemert GJ, Locke E, Morin M, Bousema T, Sauerwein RW, Long CA, Dechering KJ. An inter-laboratory comparison of standard membrane-feeding assays for evaluation of malaria transmission-blocking vaccines. Malaria Journal. 2016;15:463. doi: 10.1186/s12936-016-1515-z. [DOI] [PMC free article] [PubMed] [Google Scholar]
  21. Ogwang C, Kimani D, Edwards NJ, Roberts R, Mwacharo J, Bowyer G, Bliss C, Hodgson SH, Njuguna P, Viebig NK, Nicosia A, Gitau E, Douglas S, Illingworth J, Marsh K, Lawrie A, Imoukhuede EB, Ewer K, Urban BC, Hill AVS, Bejon P, MVVC group Prime-boost vaccination with chimpanzee adenovirus and modified vaccinia ankara encoding TRAP provides partial protection against Plasmodium falciparum infection in Kenyan adults. Science Translational Medicine. 2015;7:286re5. doi: 10.1126/scitranslmed.aaa2373. [DOI] [PMC free article] [PubMed] [Google Scholar]
  22. N'Guessan R, Ngufor C, Kudom AA, Boko P, Odjo A, Malone D, Rowland M. Mosquito nets treated with a mixture of chlorfenapyr and alphacypermethrin control pyrethroid resistant Anopheles gambiae and Culex quinquefasciatus mosquitoes in West Africa. PLoS One. 2014;9:e87710. doi: 10.1371/journal.pone.0087710. [DOI] [PMC free article] [PubMed] [Google Scholar]
  23. Papaspiliopoulos O, Roberts GO, Sköld M. A general framework for the parametrization of hierarchical models. Statistical Science. 2007;22:59–73. doi: 10.1214/088342307000000014. [DOI] [Google Scholar]
  24. Remarque EJ, Roestenberg M, Younis S, Walraven V, van der Werff N, Faber BW, Leroy O, Sauerwein R, Kocken CH, Thomas AW. Humoral immune responses to a single allele PfAMA1 vaccine in healthy malaria-naïve adults. PLoS One. 2012;7:e38898. doi: 10.1371/journal.pone.0038898. [DOI] [PMC free article] [PubMed] [Google Scholar]
  25. Rosenberg R. Malaria: some considerations regarding parasite productivity. Trends in Parasitology. 2008;24:487–491. doi: 10.1016/j.pt.2008.07.009. [DOI] [PubMed] [Google Scholar]
  26. RTSS Clinical Trials Partnership Efficacy and safety of RTS,S/AS01 malaria vaccine with or without a booster dose in infants and children in africa: final results of a phase 3, individually randomised, controlled trial. The Lancet. 2015;386:31–45. doi: 10.1016/S0140-6736(15)60721-8. [DOI] [PMC free article] [PubMed] [Google Scholar]
  27. Sauerwein RW, Richie TL. Malaria vaccines getting close to clinical reality. Vaccine. 2015;33:7423–7424. doi: 10.1016/j.vaccine.2015.10.092. [DOI] [PubMed] [Google Scholar]
  28. Schwartz L, Brown GV, Genton B, Moorthy VS. A review of malaria vaccine clinical projects based on the WHO rainbow table. Malaria Journal. 2012;11:11. doi: 10.1186/1475-2875-11-11. [DOI] [PMC free article] [PubMed] [Google Scholar]
  29. Seder RA, Chang LJ, Enama ME, Zephir KL, Sarwar UN, Gordon IJ, Holman LA, James ER, Billingsley PF, Gunasekera A, Richman A, Chakravarty S, Manoj A, Velmurugan S, Li M, Ruben AJ, Li T, Eappen AG, Stafford RE, Plummer SH, Hendel CS, Novik L, Costner PJ, Mendoza FH, Saunders JG, Nason MC, Richardson JH, Murphy J, Davidson SA, Richie TL, Sedegah M, Sutamihardja A, Fahle GA, Lyke KE, Laurens MB, Roederer M, Tewari K, Epstein JE, Sim BK, Ledgerwood JE, Graham BS, Hoffman SL, VRC 312 Study Team Protection against malaria by intravenous immunization with a nonreplicating sporozoite vaccine. Science. 2013;341:1359–1365. doi: 10.1126/science.1241800. [DOI] [PubMed] [Google Scholar]
  30. Sherrard-Smith E, Churcher TS, Upton LM, Sala KA, Zakutansky SE, Slater HC, Blagborough AM, Betancourt M. A novel model fitted to multiple life stages of malaria for assessing efficacy of transmission-blocking interventions. Malaria Journal. 2017;16:137. doi: 10.1186/s12936-017-1782-3. [DOI] [PMC free article] [PubMed] [Google Scholar]
  31. Sinden RE, Dawes EJ, Alavi Y, Waldock J, Finney O, Mendoza J, Butcher GA, Andrews L, Hill AV, Gilbert SC, Basáñez MG. Progression of plasmodium berghei through anopheles stephensi is density-dependent. PLoS Pathogens. 2007;3:e195–16. doi: 10.1371/journal.ppat.0030195. [DOI] [PMC free article] [PubMed] [Google Scholar]
  32. Singh SK, Thrane S, Janitzek CM, Theander TG, Theisen M, Salanti A, Sander AF, Sander AF. Improving the malaria transmission-blocking activity of a Plasmodium falciparum 48/45 based vaccine antigen by SpyTag/SpyCatcher mediated virus-like display. Vaccine. 2017;35:3726–3732. doi: 10.1016/j.vaccine.2017.05.054. [DOI] [PubMed] [Google Scholar]
  33. Stura EA, Satterthwait AC, Calvo JC, Stefanko RS, Langeveld JP, Kaslow DC. Crystallization of an intact monoclonal antibody (4B7) against plasmodium falciparum malaria with peptides from the Pfs25 protein antigen. Acta Crystallographica Section D Biological Crystallography. 1994;50:556–562. doi: 10.1107/S0907444994001782. [DOI] [PubMed] [Google Scholar]
  34. Talaat KR, Ellis RD, Hurd J, Hentrich A, Gabriel E, Hynes NA, Rausch KM, Zhu D, Muratova O, Herrera R, Anderson C, Jones D, Aebig J, Brockley S, MacDonald NJ, Wang X, Fay MP, Healy SA, Durbin AP, Narum DL, Wu Y, Duffy PE. Safety and immunogenicity of Pfs25-EPA/Alhydrogel, a transmission blocking vaccine against plasmodium falciparum: an open label study in malaria naïve adults. PLoS One. 2016;11:e0163144. doi: 10.1371/journal.pone.0163144. [DOI] [PMC free article] [PubMed] [Google Scholar]
  35. Stan Development Team . Stan Development Team; 2017. http://mc-stan.org/ [Google Scholar]
  36. Tiono AB, Pinder M, N'Fale S, Faragher B, Smith T, Silkey M, Ranson H, Lindsay SW. The AvecNet trial to assess whether addition of Pyriproxyfen, an insect juvenile hormone mimic, to long-lasting insecticidal mosquito nets provides additional protection against clinical malaria over current best practice in an area with pyrethroid-resistant vectors in rural burkina faso: study protocol for a randomised controlled trial. Trials. 2015;16:113. doi: 10.1186/s13063-015-0606-4. [DOI] [PMC free article] [PubMed] [Google Scholar]
  37. Tran TM, Portugal S, Draper SJ, Crompton PD. Malaria vaccines: moving forward after encouraging first steps. Current Tropical Medicine Reports. 2015;2:1–3. doi: 10.1007/s40475-015-0041-3. [DOI] [PMC free article] [PubMed] [Google Scholar]
  38. Upton LM, Brock PM, Churcher TS, Ghani AC, Gething PW, Delves MJ, Sala KA, Leroy D, Sinden RE, Blagborough AM. Lead clinical and preclinical antimalarial drugs can significantly reduce sporozoite transmission to vertebrate populations. Antimicrobial Agents and Chemotherapy. 2015;59:490–497. doi: 10.1128/AAC.03942-14. [DOI] [PMC free article] [PubMed] [Google Scholar]
  39. VanderWeele TJ, Knol MJ. A tutorial on interaction. Epidemiologic Methods. 2014;3:33–72. doi: 10.1515/em-2013-0005. [DOI] [Google Scholar]
  40. Walker PG, Griffin JT, Ferguson NM, Ghani AC. Estimating the most efficient allocation of interventions to achieve reductions in Plasmodium falciparum malaria burden and transmission in Africa: a modelling study. The Lancet Global Health. 2016;4:e474–e484. doi: 10.1016/S2214-109X(16)30073-0. [DOI] [PubMed] [Google Scholar]
  41. White MT, Bejon P, Olotu A, Griffin JT, Riley EM, Kester KE, Ockenhouse CF, Ghani AC. The relationship between RTS,S vaccine-induced antibodies, CD4⁺ T cell responses and protection against plasmodium falciparum infection. PLoS ONE. 2013;8:e61395. doi: 10.1371/journal.pone.0061395. [DOI] [PMC free article] [PubMed] [Google Scholar]
  42. World Health Organization World malaria report 2017. Geneva. 2017 http://apps.who.int
  43. Wu Y, Ellis RD, Shaffer D, Fontes E, Malkin EM, Mahanty S, Fay MP, Narum D, Rausch K, Miles AP, Aebig J, Orcutt A, Muratova O, Song G, Lambert L, Zhu D, Miura K, Long C, Saul A, Miller LH, Durbin AP. Phase 1 trial of malaria transmission blocking vaccine candidates Pfs25 and Pvs25 formulated with montanide ISA 51. PLoS ONE. 2008;3:e2636. doi: 10.1371/journal.pone.0002636. [DOI] [PMC free article] [PubMed] [Google Scholar]

Decision letter

Editor: Urszula Krzych1

In the interests of transparency, eLife includes the editorial decision letter and accompanying author responses. A lightly edited version of the letter sent to the authors after peer review is shown, indicating the most substantive concerns; minor comments are not usually included.

Thank you for submitting your article "Synergy in anti-malarial pre-erythrocytic and transmission-blocking antibodies is achieved by reducing parasite density" for consideration by eLife. Your article has been reviewed by three peer reviewers, and the evaluation has been overseen by a Reviewing Editor and Wendy Garrett as the Senior Editor. The reviewers have opted to remain anonymous.

The reviewers have discussed the reviews with one another and the Reviewing Editor has drafted this decision to help you prepare a revised submission.

Summary:

The manuscript by Sherrard-Smith et al. addresses an important question in malaria vaccine development, namely the impact of multistage vaccination approaches, e.g., pre-erythrocytic (PEV) and transmission blocking (TBV), in various transmission settings on the overall malaria infection. The paper is commendable for being cross-disciplinary (i.e. mouse experiments and modelling) and for its clarity of presentation. Figure 1 neatly provides an overview of the raw data then Figure 2 with contains the essence of the modelling output. The observation that PEV + TBV is synergistic, and specifically through reducing sporozoite counts thus giving imperfect PEVs a better chance to work is well supported for this model set up. This conclusion has been inferred from theoretical models before, and this is the first demonstration using laboratory data. The manuscript is well written, and the study design clearly laid out and well executed.

Essential revisions:

There are a few issues that the authors need to address before the manuscript is considered for an acceptance in eLife.

1) Please consider performing additional experiments that would also include varying PEV efficacy. Should you consider that such experiments would not be interesting, please justify your reason(s).

2) The other revisions concern expansions or explanations of the following points:

a) Concerning the relevance of synergy, it would be assumed that a highly efficacious PEV or TBV will not require synergy and it is only the 50% TBV where the effect is really noticeable.

b) Expand on the applicability of the murine population model to human vaccine trials and particularly how would the variabilities in human transmission be built into this assay or modeled from this populations assay.

c) Considering situations that commonly exists in the field and that do impact transmission, e.g., vaccine non-responders or a super-transmitter owing to a high oocyct counts, comment how such situations would impact the model, especially since previous preclinical work has not translated to human results.

d) Please explain the selection of the three different efficacies for TBV alone. Comment on the prevalence and the oocyst counts in the control group and the variations from experiment to experiments.

e) Finally, how could polymorphisms of TBV and PEV antigen vaccine candidates encountered in the field be accounted for in the murine population assay and how that may impact your results.

eLife. 2018 Jun 19;7:e35213. doi: 10.7554/eLife.35213.013

Author response

Essential revisions:

There are a few issues that the authors need to address before the manuscript is considered for an acceptance in eLife.

1) Please consider performing additional experiments that would also include varying PEV efficacy. Should you consider that such experiments would not be interesting, please justify your reason(s).

We agree with the reviewers that having multiple TBV doses would make the manuscript more symmetrical and exhaustive. Having seriously considered the inclusion of alternative PEV doses we feel that these experiments are beyond the scope of this piece of work for a range of reasons.

Firstly, the series of experiments described here were designed to examine the potential synergy in anti-malarial pre-erythrocytic and transmission-blocking antibodies. The PEV dose was chosen to approximately match the efficacy of RTS,S, the only malaria vaccine to have been tested in a Phase III trial. The work was intended to provide the evidence-base for why development of a partially effective TBV would be beneficial for malaria control. This was necessary as a TBV provides no direct protection to the recipient and must rely solely on community protection, something that is complex and very challenging to measure in controlled human settings. It is hoped that future generation PEVs might have a higher efficacy, the rational for investing in this additional efficacy is self-evident because the more efficacious the vaccine the more personal protection it provides. The main reason for attempting this work is that the indirect nature of how effective TBVs might be if combined with PEVs means that the outcome of using both vaccine is less obvious and potentially less predictable.

Secondly, although evidently of interest, we consider that other examinations of PEV efficacy could be more relevant and timely to public health settings than a relatively simple examination of a lower or higher static PEV efficacy. RTS,S-induced antibody concentration (and efficacy) is known to decay relatively quickly, and coverage is expected to be lower than the 100% examined in this manuscript. In the future, rather than a simple examination of a lower/higher than 50% PEV efficacy, we are interested in looking at the impact of “decaying” vaccine efficacy over time, and in examining multiple vaccine coverages (i.e. number of individuals immunized). We strongly see this as a distinct piece of work rather than an addition to the current manuscript. Additionally, we consider the experiments presented here to be exceptionally timely considering the current status of the vaccine development pipeline, and the observed findings from current efficacy trials in the field.

Finally, financially and logistically conducting these experiments is not a simple matter and is not immediately feasible. Each experiment takes approximately 165 days and requires the use of 125 mice. The addition of an additional PEV dose would require a minimum of 2 additional separate population experiments (PEV 65% vs PEV 65% + TBV 50%). An exhaustive examination of all doses (3 TBV + 3 PEV) would require an additional 7 experiments equating to over 875 mice. Any additional experiments would require further funding and time that is beyond our capacity at present. The ethical necessity for the experiments would also require some consideration given the points below.

2) The other revisions concern expansions or explanations of the following points:

a) Concerning the relevance of synergy, it would be assumed that a highly efficacious PEV or TBV will not require synergy and it is only the 50% TBV where the effect is really noticeable.

The reviewers are correct in stating that the 85% TBV (alone) treatment performed to the same level as the combination dose 85% TBV + 50% PEV, indicating that in this situation the high dose TBV was sufficient to eliminate the parasite. In this setting there was no necessity for the PEV or synergy to eliminate the parasite because the 85% achieves this alone. Nevertheless, this is unlikely to be the case in high transmission field settings as population size will be larger, vaccine coverage will be less than 100%, antibody concentration will likely decay relatively quickly, and human migration will mean cases are imported from outside the vaccinated area. Transmission dynamics mathematical models indicate that a single highly efficacious vaccine alone will be insufficient to eliminate the parasite in all settings, so control will always benefit from any synergistic interaction. We hypothesise that synergism will still be happening in 85% TBV + 50% PEV group and that, on average, the parasite would have been eliminated faster than in the 85% TBV group alone. The population assay is not sensitive enough to detect this subtle difference in control though it may be relatively important in real life-settings and could make the difference between parasite elimination and disease persistence. We have added the following to the Discussion section.

“The greatest synergy was observed in the lower TBV dose group though it is likely to operate across all TBV and PEV doses when vaccine reduces parasite density but fails to clear infection from host or vector. The 85% TBV dose administered alone eliminated the parasite over a single generation without the action of the PEV so there was no opportunity to show synergy. A 100% efficacious PEV or TBV would not require augmenting with an alternative vaccine though their efficacy is still likely to drop over time as antibodies decay so combining highly effective vaccine may still be advantageous depending on the relative rates of antibody loss.”

b) Expand on the applicability of the murine population model to human vaccine trials and particularly how would the variabilities in human transmission be built into this assay or modeled from this populations assay.

The experiment was designed to capture a range of transmission intensities simulated by using multiple mosquito bites per mouse (1, 2, 5 and 10 bites per mouse). The statistical approach used here was designed specifically to encompass this experimental design, account for high parasite over-dispersion and allow the impact of vaccine-induced antibodies on parasite density to be assessed. The population assay design meant that transmission intensity varied between groups of mice not within the same group. Transmission dynamics of malaria in the field suggest substantial within population heterogeneity in transmission as some people are bitten substantially more than others. Within population heterogeneity could be included within the mouse population assay to further investigate the impact in a control laboratory setting.

It is currently unclear how a TBV would be evaluated in humans under natural conditions. It would be possible to repeat the experimental design but using groups of humans instead of groups of mice though the feasibility and the ethics of the experiment would need to be thoroughly assessed. To investigate the synergy regulated by parasite density hypothesis within a standard human Phase III RCT would require multiple repeat measures of the density of infections in mosquitoes and people monitored during the trial. The work presented here could support the design of appropriately powered RCTs to fully assess the impact of combining vaccine components with alternative mechanisms of action.

Whilst the murine system described here uses P. berghei, the PEV component used targets CSP, the key antigen within RTS,S. Thus, the mechanism of action of the PEV antibodies administered i.v is matched to the antibody component of the RTS,S vaccine. For the TBV component, the P. berghei strainused here is genetically modified to express the human TBV candidate, P. falciparum P25 (Pfs25) in place of its P. berghei counterpart.Thus, a proven anti-falciparum TBV mAb (4B7) can be used directly within this model. This gives enhanced confidence that the synergistic impact measured would be reflected in human data (were it available). Of course, mice are not human and P. berghei is not P. falciparum. The use of model systems to examine malarial transmission is clearly necessary within multiple circumstances. The value of these studies is undoubtedly to examine the relationship between multiple anti-malarial antibody moieties, parasitic density, and ability to achieve elimination in a system that is tractable, and where these experiments are technically and ethically possible. Following the establishment of these basic dynamics in model systems, these findings should be used to inform studies with human malarial parasites in the future.

We have updated the Discussion section:

“Whilst the murine system uses P. berghei, the mechanism of action of the PEV antibodies administered is matched to the antibody-based mechanism of the RTS,S vaccine, i.e. sporozoite invasion of the liver is inhibited by the presence of CSP-targeted antibodies in mice both in vivo and ex vivo (Grüner et al., 2003). The P. berghei strain used here is genetically modified to express the human TBV candidate, P. falciparum P25 (Pfs25), in place of its P. berghei counterpart. Thus, a proven anti-falciparum TBV mAb (4B7) can be used directly within this model.

In addition, we have added the following to the Discussion section (also in response to the question below).

“The epidemiological importance of any synergistic interaction between vaccine types in the field is hard to predict and will depend on many confounding factors such as human immunity, drug treatment, vector susceptibility, antigen escape, amongst others. Transmission is likely to be highly heterogeneous, caused by factors such as vaccine non-responders and super-transmitting hosts. The impact of different types of heterogeneity can be investigated under controlled laboratory scenarios using the murine population assay, varying the vaccinated coverage, antibody dose and changing biting heterogeneity within a population. This could help understand the relative importance of these different heterogeneities and could be used to support the design of appropriately powered Phase III trials (or alternative trial designs) to fully assess the impact of combining vaccine components with alternative mechanisms of action.”

c) Considering situations that commonly exists in the field and that do impact transmission, e.g., vaccine non-responders or a super-transmitter owing to a high oocyct counts, comment how such situations would impact the model, especially since previous preclinical work has not translated to human results.

We agree that there will be greater uncertainty in field trials because so many (potentially undetectable and unmeasurable) covariates are impacting on transmission. Nevertheless, we would expect to observe some synergy from partially effective vaccines given the murine experimental results. We would argue that the population assay provides a powerful tool to help explain why epidemiological characteristics (such as heterogeneity in transmission) might influence intervention effectiveness and these results might feed into why pre-clinical work might not translate into human results as highlighted by the reviewer. In light of this we are currently investigating incomplete coverage of hosts using this model. This is posited to be equivalent to non-responders or less than 100% vaccine coverage.

We have added the following to the Discussion section:

“The epidemiological importance of any synergistic interaction between vaccine types in the field is hard to predict and will depend on many confounding factors such as human immunity, drug treatment, vector susceptibility, antigen escape, amongst others. Transmission is likely to be highly heterogeneous caused by factors such as vaccine non-responders and super-transmitting hosts. The impact of different types of heterogeneity can be investigated under controlled laboratory scenarios using the murine population assay, varying the vaccinated coverage, antibody dose and changing biting heterogeneity with a population. This could help understand the relative importance of these different heterogeneities and could be used to support the design of appropriately powered Phase III trials (or alternative trial designs) to fully assess the impact of combining vaccine components with alternative mechanisms of action.”

d) Please explain the selection of the three different efficacies for TBV alone. Comment on the prevalence and the oocyst counts in the control group and the variations from experiment to experiments.

In terms of PEVs, the most advanced malaria vaccine achieved just a 36.3% efficacy in early trials (and at the time of designing the present work). There has been much debate over the approval of this vaccine. Given this, the next malaria vaccine to be developed may well need to perform better. We considered 50% as a lower limit. Similarly, producing a highly effective (TBV) vaccine will be undoubtedly challenging in reality so we capped the upper limit to 85% within this study. The lowest TBV efficacy of 50% was chosen under the premise that a TBV of <50% reduction in oocyst prevalence would not practically be considered for release as part of a vaccine development pipeline. 65% was chosen as an intermediate efficacy point. In term of oocyst counts in control groups and experimental variation while titrating doses of 4B7, a series of transfused mAb-4B7 doses were tested in multiple (n = 6) direct feeding assays, each with an individual control. The statistical analysis used here is expressly designed/chosen to examine experimental variation in non-parametric oocyst counts over multiple experiments over a range of transmission settings (see Churcher et al., 2012, Blagborough et al., 2013, Upton et al., 2015, Churcher at al., 2017 and Sherrard-Smith et al., 2017, for more information).

We have added in subsection “Transmission-blocking vaccine surrogate: Monoclonal antibody 4B7 (mAb-4B7). The TBV”:

“Given the severity of malaria, the World Health Organization (WHO), the Strategic Advisory Group of Experts (SAGE) on Immunization and the Malaria Policy Advisory Committee (MPAC) recommended the RTS,S vaccine could be implemented in pilot countries in October 2015 (http://www.malariavaccine.org/malaria-and-vaccines/first-generation-vaccine/rtss, accessed 04/04/2018) when the vaccine was demonstrating relatively low efficacies of just 36.3% in children aged 5 to 17 months (RTSS Clinical Trials Partnership 2015). These TBV doses were chosen to bridge a range of malaria vaccine efficacies that might be acceptable by WHO, SAGE and MPAC.”

e) Finally, how could polymorphisms of TBV and PEV antigen vaccine candidates encountered in the field be accounted for in the murine population assay and how that may impact your results.

When considering the overall practical impact of all antimalarial vaccines, and, more broadly, all interventions, (bloodstage, pre-erythrocytic and transmission blocking) we fully agree that the impact of polymorphisms and the associated possibility of pathogen escape must be considered. The interventions (both PEV and TBV) used here are monoclonal antibodies against both CSP and P25 respectively. As such, the interventions utilized target only a very limited number of epitopes with pre-proven efficacy. Therefore, the experimental design here, although well suited to examine parasitic density, is not optimised for the emergence of single or multiple polymorphisms over time. When considering the use of vaccines in the field, it is likely that the introduction of polymorphisms will reduce overall vaccine efficacy/effectiveness. In the future, complimentary studies that examine the potential impact of this could be designed using this system, and administration of vaccines with a broader epitope range, followed by sequential transmission of parasites from mouse-to-mosquito-to-mouse. Specific polymorphism could be introduced by transgenesis, or screening for “naturally” occurring spontaneous polymorphism could be performed, in parallel with constant monitoring of efficacy over time. However, this is outside the remit of the current study.

We have highlighted the possibility of antigen escape in the Discussion section.

“The epidemiological importance of any synergistic interaction between vaccine types in the field is hard to predict and will depend on many confounding factors such as human immunity, drug treatment, vector susceptibility, antigen escape, amongst others.”

Associated Data

    This section collects any data citations, data availability statements, or supplementary materials included in this article.

    Supplementary Materials

    Table 1—source data 1. The raw data used for analysis.
    elife-35213-table1-data1.xlsx (112.7KB, xlsx)
    DOI: 10.7554/eLife.35213.006
    Transparent reporting form
    elife-35213-transrepform.pdf (883.7KB, pdf)
    DOI: 10.7554/eLife.35213.010

    Data Availability Statement

    All data generated or analysed during this study are included in the manuscript and supporting files.

    Articles from eLife are provided here courtesy of eLife Sciences Publications, Ltd

    RESOURCES