key: cord-0708495-r64to6fv
authors: Mohsen, Mona O.; Rothen, Dominik; Balke, Ina; Martina, Byron; Zeltina, Vilija; Inchakalody, Varghese; Gharailoo, Zahra; Nasrallah, Gheyath; Dermime, Said; Tars, Kaspars; Vogel, Monique; Zeltins, Andris; Bachmann, Martin F.
title: Neutralization of MERS coronavirus through a scalable nanoparticle vaccine
date: 2021-08-24
journal: NPJ Vaccines
DOI: 10.1038/s41541-021-00365-w
sha: a8d8f32bfc2afc69df0ca2883ac15ac2472ea713
doc_id: 708495
cord_uid: r64to6fv

MERS-CoV continues to cause human outbreaks, so far in 27 countries worldwide following the first registered epidemic in Saudi Arabia in 2012. In this study, we produced a nanovaccine based on virus-like particles (VLPs). VLPs are safe vaccine platforms as they lack any replication-competent genetic material, and are used since many years against hepatitis B virus (HBV), hepatitis E virus (HEV) and human papilloma virus (HPV). In order to produce a vaccine that is readily scalable, we genetically fused the receptor-binding motif (RBM) of MERS-CoV spike protein into the surface of cucumber-mosaic virus VLPs. The employed CuMV(TT)-VLPs represent a new immunologically optimized vaccine platform incorporating a universal T cell epitope derived from tetanus toxin (TT). The resultant vaccine candidate (mCuMV(TT)-MERS) is a mosaic particle and consists of unmodified wild type monomers and genetically modified monomers displaying RBM, co-assembling within E. coli upon expression. mCuMV(TT)-MERS vaccine is self-adjuvanted with ssRNA, a TLR7/8 ligand which is spontaneously packaged during the bacterial expression process. The developed vaccine candidate induced high anti-RBD and anti-spike antibodies in a murine model, showing high binding avidity and an ability to completely neutralize MERS-CoV/EMC/2012 isolate, demonstrating the protective potential of the vaccine candidate for dromedaries and humans.

Over the past two decades, different highly pathogenic coronaviruses caused several major outbreaks as seen with severe acute respiratory syndrome (SARS) The WHO MERS report, published on January 2020 has recorded a total number of 2519 confirmed cases including 866 associated deaths (case-fatality rate of 34.3%) worldwide. The majority of the cases were reported in Saudi Arabia. Death occurred in patients between 45-85 years with comorbidities and no changes in the demographic and epidemiological characteristics have been reported when compared to the periods in 2014-2020 3 . Interestingly, a recent case series study has reported that 12% of the total numbers of MERS-infected cases admitted to the intensive care unit (ICU) (from March 14, 2020 to October 19, 2020) showed coinfection with SARS-CoV-2 4 . This study raises new concerns of the possibility of interaction between both coronaviruses.

Similar to other coronaviruses, MERS-CoV is a zoonotic virus originating from bats, which probably serve as natural reservoirs (Lu et al., 2015) , while dromedary camels most likely are intermediate hosts where the virus, however, remains endemic and causes mild symptoms similar to seasonal CoVs in humans (Abdulaziz N. Alagaili et al., 2015) . Transmission of MERS-CoV among humans is considered rare but yet very possible. Due to the high mortality rate of MERS virus (∼25-35%), the WHO declared the need for effective countermeasures such as vaccines for dromedaries as well as for humans. Indeed, this human to human transmissible disease represents a major threat and should gain political and public health attention before a next major outbreak.

Coronaviruses infect host cells via their spike glycoprotein which consists of S1 and S2 subunits. The S1 of MERS-CoV is encoded by amino acids (a.a.) 376-606 and contains the receptorbinding domain (RBD) that is composed of a core subdomain and a receptor-binding motif (RBM; a.a. 484-567). The RBM is the main domain that interacts with the DPP4 receptor and facilitates viral entry into target cells 5, 6 . After attaching to the cell surface, peptidases from the host cleave the S proteins, exposing the fusion peptide located in the S2 subunit. Such process leads to fusion of the viral and host cell membranes which enables the viral genome to enter the host cell. As for many other viruses, fusion mostly occurs in endosomes causing the release of the viral genome into the host cytosol. Finally, the viral RNA becomes available for translation and replication, resulting in assembly and packaging of new viral particles which are released from the cell 7 . Accordingly, the RBD and in particular the RBM domain may be considered the principal target against MERS-CoV for vaccine development.

Previous approaches for developing MERS-CoV vaccines included DNA vaccines, viral vectors, protein-based platforms or inactivated viruses 8 . The delivery of MERS-CoV S antigen by means of DNA vaccination 9 , viral vectors (modified vaccinia Ankara MVA or adenovirus) 10,11 , nanoparticles 12 or RBD-based subunit vaccines 13 have proved efficacy in preclinical models against MERS-CoV. Several vaccines are currently in phase I clinical trials. Despite the promising results and active research on this area, neither antiviral drugs nor vaccines have been approved for veterinary or medical use against MERS 14 .

Virus-like particles (VLPs) are nanoscale multiprotein particles that mimic real viruses. In comparison to inactivated or liveattenuated vaccine platforms, VLP-based vaccines are capable of inducing a robust humoral immune response without the risk of reversion to virulence 15 and do not require BSL-3 facility. Due to their nano-size dimensions, they readily reach draining lymph nodes where they induce a strong immune response 16, 17 . Such rapid draining kinetics improves the exposure of B cells to native VLPs and reduces potentially systemic inflammatory responses 18 . The traditional VLP platform has been used in several marketed vaccines against Hepatitis B Virus (HBV), Hepatitis E Virus (HEV), Human Papilloma Virus (HPV) as well as malaria 19 .

Cucumber mosaic virus-like particles (CuMV-VLPs) are derived from a plant virus. We have recently developed an immunologically optimized platform based on CuMV-VLPs, by incorporating a universal tetanus toxin (TT), a T helper (T H ) cell epitope into the particle (CuMV TT -VLPs) 20 . This results in enhanced B cell / T H cell interactions, especially important for elderly people and individuals with weak immune responses. This platform has reached several proofs of concepts in various animal species (reviewed in 20, 21 ) . Furthermore, our newly developed vaccine platform is selfadjuvanted with prokaryotic ssRNA which is packaged within VLPs during the expression and assembly process in E. coli. The selfpackaged adjuvant serves as TLR7/8 ligand and promotes the activation of antigen-presenting cells (APCs) and B cells [22] [23] [24] [25] .

Several methods can be used to display antigen epitopes on the surface of VLPs; these methods include chemical coupling and genetic fusion techniques. In our previous studies we used chemical coupling strategies such as SMPH or Cu-free click chemistry cross-linkers [26] [27] [28] . In this study, we have chosen to genetically insert the viral antigen into the VLP protein, enabling future GMP-compatible production at very large scale at low cost. The size of the engineered mCuMV TT -MERS particles are in the nanoscale of ∼40-50 nm and densitometric analysis suggests an approximate 40% incorporation of RBM. On the surface of the VLPs, RBM exhibits the right conformation as demonstrated by binding of the viral receptor DPP4. Here we show that our new vaccine is immunogenic in murine models and induces high RBD and spike specific -antibody titers which are capable of blocking the replication of MERS-CoV/EMC/2012 isolate in vitro.

We have used our immunologically optimized plant-derived cucumber-mosaic VLPs (CuMV TT -VLPs) to develop a mCuMV TT -MERS nanovaccine candidate. The icosahedral T = 3 CuMV TT -VLPs are identical to the parent VLPs where subunits A are arranged in pentamers and subunits B/C are arranged in hexamers 25 . CuMV TT -VLPs incorporate a tetanus toxin (TT) epitope which is a universal T cell epitope binding to essentially all HLA-DR molecules. The incorporated TT epitope is displayed at the interior surface of the particles, allowing the VLPs to self-assemble without altering their icosahedral geometry or interfering with epitopes to be displayed on the exterior surface 20, 29 . Furthermore, displaying the TT epitope on the interior surface of the particle prevents interference with TT-specific antibodies. TT-epitope incorporation is believed to improve the immune response specifically in aged people due to enhanced interaction between TT-specific T H cells and epiotpe specific B cells, and is based on the fact that pre-existing immunity to TT epitope is broad in humans due to extensive vaccination programs. We have incorporated the coding sequencine of the receptor-binding motif (RBM; a.a. 484-566) of MERS-CoV protein into CuMV TT nanoparticles. The RBM domain has been selected based on previous studies on SARS-CoV-2, where RBM proved to be a potent vaccine epitope 30, 31 .

The vaccine candidate was engineered as a mosaic particle where unmodified wild-type monomers and genetically modified monomers (incorporating RBM) assemble together forming a VLP (Fig. 1a) . Purification of mCuMV TT -MERS was carried out using sucrose gradient (Fig. 1b) . The unmofidied monomer has a size of~28 kD while the ones incorporating RBM have an apparent size of~42 kDA as shown in SDS-PAGE (Fig. 1c) . Furthermore, the production of mCuMV TT -MERS in E. coli system allowed spontaneous packaging of ssRNA which serve as toll-like receptor (TLR) 7/ 8 agonist. We have also tested the stability of the vaccine candidate and the results indicate that the platform is thermostable at 4°C for more than a year and for about a month at RT (Fig. 1d) . The size of the engineered mCuMV TT -MERS particles is 40-50 nm. Densitometric analysis suggests an approximate 40% incorporation of RBM. As each VLP contains 180 capsid protein (CP) subunits, 40% results in~70 RBM antigen-containing CuMV TT -CP molecules per 1 VLP ( Fig. 1e and Video 1). Dynamic light scattering revealed a homogenous and uniform peak of hydrodynamic radius (R H ) of~94 nm (Fig. 1f) ; the observed peak is larger than the expected size due to water molecules surrounding the VLPs. Electron microscopy imaging confirms the assembly of icosahedral particles and indicated no signs of VLP aggregation following expression in E. coli (Fig. 1g ).

To confirm the antigenicity of mCuMV TT -MERS as well as the correct folding and confirmation of RBM displayed on the particle's surface, we performed a receptor binding assay. To this end, the human receptor DPP4 was coated on ELISA plate. mCuMV TT -MERS vaccine was added, in parallel to CuMV TT as a control. Anti-CuMV TT antibodies were used as a secondery antibody to detect receptor bound VLPs. The results revealed that mCuMV TT -MERS can bind to DPP4 receptor indicating correct folding of RBM on the surface of the VLP while the control did not show any binding (Fig. 2) .

The immunogenicity and the induction of a humoral immune response in murine models upon vaccination with mCuMV TT -MERS was examined by ELISA. BALB/c mice were primed s.c. with 100 μg CuMV TT as a control or with mCuMV TT -MERS vaccine candidate without any adjuvant. A booster dose was given 28 days later. Mice were bled on a weekly basis and terminally bled on day 49 as illustrated in Fig. 3a . Total IgG was measured against RBD as well as against spike protein of MERS-CoV. RBD-specific IgG antibodies were detected as early as seven days post priming in the group vaccinated with mCuMV TT -MERS. The induced response against RBD increased ∼10-fold following priming and reached the peak one week after the booster dose (Fig. 3b, c) . The response against spike protein was somewhat delayed compared to the response against RBD protein. Nevertheless, an~100-fold increase in IgG titer was detected three weeks after priming on day 21 and further increased following the booster dose (Fig. 3d, e) . No RBD or spike specific antibodies were detected prior to vaccination. mCuMV TT -MERS vaccine induces RBD and spike-specific IgG subclasses as well as isotype switching to IgA We next evaluated the ability of the engineered vaccine candidate to induce IgG subclasses and IgA using the sera collected at day 49. To this end, ELISA plates were coated with RBD or spike proteins of MERS-CoV. The results showed that mCuMV TT -MERS vaccination induces the production of all RBD-specific IgG subclasses (IgG1, IgG2a, IgG2b and IgG3) dominated by IgG1 and IgG2a (Fig. 4a, b) . IgG subclasses could also be detected against the spike protein as shown in Supplementary Fig. 1 . Isotype switching to RBD-specific IgA antibodies was also induced following vaccination with mCuMV TT -MERS (Fig. 4c) and reached an OD 50 of greater than 1:100 (Fig. 4d) .

To further characterize the induced RBD-specific IgG antibodies, we performed avidity ELISAs using sera collected one week following the booster dose. The results showed that the mCMV TT -MERS vaccine is capable of generating high avidity antibodies (Fig. 5a ). Essentially no difference was detected between the ELISA plates treated with PBST or 7 M UREA (to eliminate low avidity antibodies) for the group vaccinated with mCuMV TT -MERS (Fig. 5b) . We also calculated the avidity index by comparing the two treated plates for the group vaccinated with mCuMV TT -MERS. The mean index was~0.6, indicating that around 60% of the total IgG antibodies are of high avidit for RBD (Fig. 5c) . The avidity of the spike-specific antibodies was also tested (Fig. 5d ). The small difference (p. 0.0327) detected between the sera treated with PBST or Urea indicate that about 30% of the generated antibodies could recognize the spike protein with high avidity (Fig. 5e, f) .

To determine whether the induced IgG antibodies can compete with the human receptor DPP4 for binding to RBD, we performed antibody competition assays using biolayer interferometry. RBD-His was immobilized onto anti-His biosensors and competitions of DPP4 to RBD was quantified as reduction in RBD binding in the presence of serum samples. As shown in Fig. 6a , sera of mice immunized with mCuMV TT -MERS were able to inhibit DPP4 binding to RBD. For comparison, sera from control mice immunized with CuMV TT alone were used. The results indicate that immunization with mCuMV TT -MERS induced anti-RBM antibodies capable of inhibiting the binding of MERS-RBD to DPP4.

To determine the neutralizing capacity of the induced antibodies, the sera were tested for their ability to prevent cytopathic effects of MERS-CoV/EMC/2012 on Vero cells in vitro (CPE-based neutralization assay). The titer is indicated as the dilution at which an inhibiting effect was visible and the cytopathic effect was fully prevented. The group vaccinated with mCuMV TT -MERS fully inhibited the cytopathic effect of the virus while the control group CuMV TT did not show any inhibition, demonstrating a strong neutralizing capacity of the induced antibodies (Fig. 6b) . 12 . The same group has tested another VLP vaccine containing MERS-CoV S, E and M proteins in rhesus macaques which also showed efficacy 32 .

In the present study, we have engineered a vaccine candidate against MERS-CoV by genetically fusing the RBM domain of MERS-CoV into our immunologically optimized VLP-platform derived from the cucumber-mosaic virus (CuMV TT -VLPs). Designing the vaccine-candidate in this study as a mosaic vaccine was an essential step to allow the formation of icosahedral T = 3 VLPs 25 . Each engineered VLP incorporates~70 RBM fused to the CP (40%).

Expression in E. coli facilitateted the packaging of bacterial ssRNA which serves as TLR7/8 ligand. Previous studies demonstrated that VLP-based vaccines are capable of inducing IL-21-independent secondery plasma cells only in the presence of TLR7/8 agonists (ssRNA). Consequently, high levels of IgG antibodies with high affinity are produced within few days after challenge 22, 33 . ssRNA packaged in VLPs polarizes the induced immune response towards T H 1 rather than T H 2, which prevents enhanced disease after viral challenge at least in preclinical models 2 . In addition, we incorporated a tetanus toxin (TT) epitope in the interior surface of our CuMV TT -VLPs. This may not necessarily affect the antibody response in mice or dromedaries as they are not pre-immunized against TT. However, the immunogenicity will be enhanced in humans due to previous tetanus vaccinations, likely helpful in elderly people and immunodeficient individuals who are known to require more immunogenic vaccines as compared to the general population. We have chosen the RBM-MERS as our vaccine target based on several grounds: (1) we found that genetically fusing the whole RBD domain of SARS-CoV-2 into VLPs hinders the assembly process of VLPs; on the other hand fusing RBM in AP205-VLPs resulted in an effective vaccine capable of neutralizing SARS-CoV-2 31 . (2) Based on previous studies for SARS-CoV-1 and 2, RBD is glycosyated and methylated. Such posttranslational modifications may be difficult to reproduce in bacteria and may result in the induction of low affinity, poorly protective antibodies. Importantly, RBM is neither glycosylated nor methylated and thus can directly interact with the human receptor MERS-DPP4. RBM is also the major target of neutralizing antibodies 34, 35 and therefore represents and ideal vaccine target. To our knowledge, we present here the first VLP-based vaccine displaying the RBM domain of MERS-CoV that can easily be produced in large amounts as it selfassembles in E. coli without the need of any further modifications.

Vaccine candidates should display antigens in an authentic native configuration in order to induce an effective B cell response 18 . Using Sandwich ELISAs, we have shown that mCuMV TT -MERS particles are able to detect and bind to the viral receptor DPP4. This confirms that the MERS RBM displayed and fused to the VLP, has the correct conformation which is important for the induction of the appropriate neutralizing antibody response.

We have not directly measured the induction of T H cells responses by our vaccine candidate, mostly because the expected effector mechanism is induction of neutralizing antibodies. In addition, the size of the RBM-domain may be too small to reliably induce a T H cell response in inbred mice. However, we have previously shown that VLP-specific T H cell responses mediate isotype-switch for B cells specific for antigens displayed on the VLPs. Furthermore, the bacterial RNA packaged in VLPs, such as CuMV TT , drive CD8 + and T H 1 responses. (44-46) .

Mouse IgG antibodies vary in their immunological, biochemical as well as physiological properties. We have previously shown that TLR7/8 triggering in B cells induces subclass switch to IgG2a and IgG2b; bacterial RNA was most efficient at triggering such responses 23, 36 . Vaccination with mCuMV TT -MERS enhanced the induction of all IgG subclasses which was dominated by IgG1 and IgG2a, other subclasses could also be detected to a much lesser extent. In addition, RNA loaded VLPs may also induce IgA responses, again in a TLR7/8 dependent manner 22, 24 . This appears particularly important for MERS-CoV and other respiratory diseases-causing viruses, such as SARS-CoV-1 and −2, as IgA may be able to neutralize the virus locally in the lung without causing inflammation, a feature that may be particularly critical in patients with high viral load. IgA is the predominant Ig isotype in the mucosal tissue and has a very important role in the defense against respiratory infections 37 . Thus, an effective vaccine against respiratory viruses should induce IgA antibodies. It is therefore of key importance that our newly developed vaccine is able to induce a significant increase in serum IgA levels. Whether the increased serum IgA levels in mice can translate to correspondingly high IgA levels in humans and the mucosa needs to be confirmed.

Testing the quality of the RBD-specific antibodies has shown high avidity binding which is a critical parameter for an effective vaccine. UREA is interfering with the antibody-antigen binding by breaking up the hydrophobic bonds. We found that~60% of the RBD specific IgG antibodies are of high avidity and bind strongly to its antigen even in the presence of UREA. Thus, RBM displayed on CuMV TT induces high avidity antibodies.

The main goal for any anti-viral vaccine is the elicitation of neutralizing antibodies which are able to directly inhibit cellular infection and provide protection from disease 38 . For MERS-CoV, most neutralizing antibodies bind to the spike glycoprotein and inhibit viral attachement to the human receptor DPP4, hence blocking viral entry and intracellular replication. Our test sera were probed for their ability to inhibit the cytopathic effect of MERS-CoV/EMC/2012 isolate on Vero cells. Indeed, sera from vaccinated mice were able to fully neutralize viral replication, showing that the vaccine is able to induce protective antibodies which can shield the host's cells from MERS-CoV infection.

Collectively, we have shown in this study that an engineered VLP-based vaccine can efficiently induce high specific anti-RBD and spike antibodies that effectively neutalize MERS-CoV. As MERS represents an immanent global threat to human health, it seems rational to further develop this vaccine candidate and make it availalbe for emergency use.

METHODS mCuMV TT -MERS vaccine candidate production, purification and analysis E. coli C2566 cells were transformed with the pETDu-CMVB3d-MERS-M-CMV TT plasmid containing RBM of MERS and the Ampicillin (Amp) resistance gene. After transformation, five individual colonies were inoculated in 4 ml 2TY (1.6% Trypton, 1.0% Yeast extract, 0.5% NaCl) with Amp (100 mg/l) and 0.1% glucose and cultured overnight at 37°C without shaking. The next day, 1 ml of the starting culture was added to 20 ml 2TY, cultivated at 30°C until an OD 600nm of 0.8 was reached and then induced with 0.2 mM IPTG and 5 mM MgCl 2 and cultivated ON at 20°C and 7 xg. After 18 h an OD 600n m of 5.20 was reached and samples for SDS-PAGE were prepared. After SDS-PAGE analysis of individual clones the 5 20 ml cultures were pooled together (100 ml in total) and the biomass was collected by centrifugation. The pellet was frozen at −20°C. To disrupt the cells, 10 ml of buffer (20 mM Tris, 5 mM EDTA, 5 mM Et-SH, 5% glycerol, 10% sucrose, pH 8.0) was added to resuspend and further treat the biomass with ultrasound (Hielscher 200, power 70%, pulse 50%, 16 min) on ice. Then, 0.5% TX-100 was added and the solution was rotated at 10 rpm overnight (ON) at 4°C without centrifugation. The solution was then centrifugated for 10 min at 15,557 xg (Eppendorf 5804) and the pellet was discarded. The soluble fraction was loaded on the top of the sucrose gradient (20-60%; in buffer containing 20 mM Tris, 2 mM EDTA, 5% glycerol, 0.5% TX-100, pH 8.0) and centrifugated in Beckman SW32 rotor for 6 h at 106,559 xg at 18°C. The gradient fractions (6 ml) were then Fig. 4 mCuMV TT -MERS vaccine induces RBD and spike-specific IgG subclasses as well as isotype switching to IgA. a RBD-specific IgG1, IgG2a, IgG2b and IgG3 titers for the groups vaccinated with CuMV TT control or mCuMV TT -MERS measured with OD 450 . b Log 10 OD 50 values (mean ± SEM) of RBD-specific IgG1, IgG2a, IgG2b and IgG3 titer for the groups vaccinated with mCuMV TT -MERS, (p value 0.0202 for IgG1 vs IgG2b, p value 0.0096 for IgG1 vs IgG3). Statistical analysis using One-way ANOVA. Control group n = 4 and vaccine group n = 4. c RBD-specific IgA titer for the groups vaccinated with CuMV TT control or mCuMV TT -MERS measured with OD 450 . d Log 10 OD 50 values (mean ± SEM) of RBD-specific IgA titer for both groups, (p value < 0.0001). Statistical analysis using Student's t test. Control group n = 5 and vaccine group n = 5. One representative of two similar experiments is shown. The value of p < 0.05 was considered statistically significant (*p < 0.01, **p < 0.001, ***p < 0.0001).

removed from the bottom of the 38 ml tube. The mCuMV TT -MERS containing fraction (40 and 50% sucrose, pooled) was diluted 1:1 with buffer (20 mM Tris, 2 mM EDTA, 5% glycerol, pH 8.0). The VLPs were sedimented using Type 70 rotor (Beckman, 183,960 xg, 4 h, 4°C). Then the pellet was dissolved ON in 2 ml of 20 mM Tris, 2 mM EDTA at 4°C. The solution was clarified by centrifugation (5 min, 16,873 xg), the clarified solution overlaid on top of the 30% sucrose "cushion" solution in 20 mM Tris, 2 mM EDTA, 0.5% TX-100, pH 8.0 The VLPs were sedimented using Beckman TLA100.3 rotor (220,050 xg, 60 min, 4°C). The pellet was solubilized in 1 ml of 20 mM Tris, 2 mM EDTA and clarified again by centrifugation (5 min, 16,873 xg). Obtained VLPs were characterized using SDS-PAGE, agarose gel, electron microscopy and dynamic light scattering. Protein concentration was determined using BCA test.

To test if the vaccine can bind the relevant human receptor DPP4, the plates were coated with 1 µg/ml of DPP4 in PBS at a volume of 50 μl/well. The plate was incubated at 4°C overnight. The plate was washed with PBS+Tween 0.01%. 50 μl/well of Superblock solution (Thermo Fisher, 37518) was added and the plate was incubated for 1 h at RT on a shaker. The blocking solution was flicked off and 50 μl of mCuMV TT -MERS or CuMV TT (control) from 1 µg/ml was added to the first row of the plate followed by 1:3 dilution. The plate was incubated for 1 h at RT then washed with PBS+Tween 0.01%. Next, 50 μl of mouse anti-CuMV TT monoclonal antibody (clone 1-1A8/ batch 2) at a concentration of 1 μg/ml was added to each well as a secondary antibody and incubated for 1 h at RT on a shaker. The plate was washed and 50 μl of the detection antibody; HRP labeled goat anti-mouse IgG Fc gamma at a dilution of 1:1000 in PBS-Casein 0.15% was added to each well. The plate was incubated for 1 h at RT. The plate was developed and OD450 reading was performed (BioTek, USA).

Wild type Balb/cOlaHsd mice were purchased from Harlan. All in vivo experiments were performed using 8-12 weeks old female mice.

All animal procedures were conducted in accordance with the Swiss Animal Act (455.109.1 -September 2008, 5th) using License No. BE70/ 2018.

Wild type Balb/cOlaHsd mice (8-12 weeks, Harlan) were vaccinated subcutaneously (s.c.) in the neck with 100 μg with either mCuMV TT -MERS vaccine or CuMV TT as a control in a volume of 100 μl without any adjuvants. The mice received a boost with an equal dose at day 28 and were terminally bled at day 56. Serum was collected on a weekly basis vial tail bleeding and the serum was isolated using Microtainer Tube (BD Biosciences, USA). . c, f Avidity index showing the percentage of high avidity RBD-and spike-specific IgG antibodies calculated with the data from (a) or (d). Statistical analysis using Student's t test. Control group n = 5 and vaccine group n = 5. One representative of 2 similar experiments is shown. The value of p < 0.05 was considered statistically significant (*p < 0.01, **p < 0.001, ***p < 0.0001).

To determine the total IgG antibody titers, ELISA Corning TM 96-Well Half-Area Plates (Fisher Scientific, USA) were coated with 1 μg/ml MERS-CoV RBD, (a.a. 367-606) (Sino Biological, USA) or MERS-CoV Spike/S1 protein S1 Subunit, (a.a. 1-725), diluted in PBS in a volume of 50 µl/well. The plates were incubated overnight at 4°C on a shaker. The next day the plates were washed with the ELISA washer (BioTek, 405 TS) with PBS-tween 0.01%. The plates were blocked using 100 μl/well PBS-Casein 0.15% and incubated at RT for 2 h on a shaker. The blocking solution was removed by flicking the plates. Serum samples were diluted 1:20 followed by 1:3 serial dilution except for the last row which was used as a negative control. The plates were incubated for 2 h at RT on the shaker. Plates were washed with PBS-tween 0.01% and secondary anti mouse IgG Fc gamma conjugated with Horse-Radish Peroxidase (Jackson Immunoresearch Cat. Nr. C840T69) (1:1000) was added 50 μl/well. The plates were incubated for another 1 h on a shaker, then washed and developed and OD450 reading was performed (BioTek, USA). Log 10 OD 50 values were calculated using GraphPad PRISM.

To assess the subclass antibody response, the same procedure was performed, except using a different secondary antibody equivalent to each subclass: Rat anti-mouse IgG1 (BD Pharmingen, Cat. To detect IgA antibodies the plates were coated with 1 μg/ml MERS-CoV RBD, (a.a. 367-606) (Sino Biological, USA) and goat anti-mouse IgA POX (ICN 55549, ID 91, 1:1000 dilution) was used as a secondary antibody. An additional step prior to serum incubation in order to deplete IgG was performed. 10 μl of Protein G beads (Invitrogen, USA) were transferred into a tube and placed into a magnet. The liquid was removed and 75.6 µl diluted sera in PBS-Casein 0.15% was added to the beads and mixed. The tube was incubated on a rotator at RT for 10 min. The tubes were placed back into the magnet and ELISA was carried out as described above.

To determine the avidity of IgG antibodies, two sets of plates were prepared. Both were coated with 1 µg/ml MERS-CoV RBD, (a.a. 367-606) (Sino Biological, USA). After serum incubation, one set of plates was washed three times for 5 min with 50 µl/well 7 M Urea in PBS+0.05% Tween 20 whereas the other set was washed with the same amount of PBS +0.05% Tween. In-between the washing steps, all the plates were washed with PBS+0.01% Tween 20 with the ELISA washer. The rest of the procedure is identical as described above.

The antibody competitive binding activities of the induced antibodies was performed on an OCTET RED96e (Fortébio) instrument which allows real-time analysis due to the shift in the wavelength of the reflected light. Anti-Penta-HIS (HIS1K, Lot 2006292, FortéBio) biosensors were first loaded into biosensor microplates and pre-hydrated in BLI assay buffer (PBS, 0.1% BSA, 0.02% Tween 20) for 10 min. 96-well microplates were loaded with 200 ml per well. The assay plate was then prepared as follows: column 1 (BLI assay buffer), column 2 (15 μg/ml MERS-CoV spike protein fragment RBD, aa267-606, diluted in 200 μl BLI assay buffer) (Sino Biological, USA), column 3 (BLI assay buffer), column 4 (pooled sera from 5 mice diluted 1:10 in BLI assay buffer, samples from control mice vaccinated with CuMV TT -VLPs alone and mice vaccinated with mCuMV TT -MERS were used, two additional biosensors were used as control, one for baseline and one without serum sample), column 5 (BLI assay buffer), column 6 (50 nM of human receptor DPP4 (Sino Biological, USA) diluted in BLI assay buffer), column 11 (Regeneration buffer, 0.1 M glycine, pH 1.5) and column 12 (neutralization buffer, BLI assay buffer).

Serum samples from day 56 were heat-inactivated for 30 min at 56°C. Subsequently, serum samples were diluted two-fold, started at 1:20 to 1:160. Then 100 TCID50 of MERS-CoV/EMC/2012 was added to each well and incubated at 37°C for 1 h. Following incubation, the mixtures were added on a monolayer of Vero cells and incubated at 37°C for an additional four days. After four days wells were inspected for presence of cytopathic effect (CPE). Titer is expressed as the highest serum dilution that fully inhibits formation of CPE. Binding of DPP4 to BLI biosensors coated with RBD-his tag is significantly reduced in the presence of mouse sera (1:10 dilution, d35) after 2nd vaccination with mCuMV TT -MERS (brown line) than with CuMV TT control (green line) or with no serum (line orange) consistent with DPP4-blocking activity. b Neutralization titers (CPE) of the groups vaccinated with CuMV TT control and mCuMV TT -MERS, p < 0.0001. Statistical analysis using Student's t test. Control group n = 10 and vaccine group n = 9. One representative of two similar experiments is shown. The value of p < 0.05 was considered statistically significant (*p < 0.01, **p < 0.001, ***p < 0.0001).

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Role of IgA in the defense against respiratory infections IgA deficient mice exhibited increased susceptibility to intranasal infection with Mycobacterium bovis BCG

Deconstructing the antiviral neutralizingantibody response: implications for vaccine development and immunity. Microbiol Mol

This work was supported by MRC-HMC (grant 29032016), Qatar National Research Fund (PDRA grant PDRA4-0118-18002) and by the Swiss National Science Foundation (SNF 310030_185114 and SNF 310030_179165). We would like to thank Prof. Daniel Speiser for his thorough editing of the paper.

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