Introduction

Neisseria meningitidis (Nm) is a leading cause of bacterial meningitis and sepsis worldwide. The strictly human pathogen causes recurrent devastating epidemics in developing countries, in particular the African sub-Saharan meningitis belt.1 In Western World countries, Nm infections occur sporadically, but outbreaks have been reported caused by hyper-invasive strains in situations of crowding2,3 and in communities with increased risk.4,5 As Nm is the only bacterial pathogen that can spread in epidemic waves, outbreaks present a significant danger for individuals with high susceptibility, that is, small children, adolescents and elderly people.6

A chief problem with invasive meningococcal disease (IMD), often characterised by meningitis and sepsis, is rapid progression. IMD can lead to death within hours,7 leaving open an extremely short window for medical intervention. Accordingly, case-fatality rates are high, exceeding 20% even in developed countries.8 Moreover, survivors often suffer from fatal sequelae like limb loss, deafness and neurologic disabilities.9 The benefit of vaccination is obvious on this background and motivated industrial companies (GSK Vaccines, Pfizer, Baxter, Sanofi-Pasteur, Serum Institute of India10) and international nonprofit organisations like PATH and WHO11,12 to invest into the development of vaccines to combat IMD and thus improve health and life conditions in afflicted regions.

Major virulence factors of Nm are the capsular polysaccharides (CPS).13 Twelve chemically different CPSs have been identified and determine the twelve Nm serogroups, of which six (NmA, -B, -C, -W, -Y and -X) account for virtually all cases of IMD.13 With the exception of NmB, where the CPS (CPSB) consists of α2,8-linked polysialic acid identical to host-expressed polysialic acid,14,15 the CPSs coupled to adjuvant proteins provide the basis for modern vaccine formulations, the so called glycoconjugate vaccines.16 Currently, mono- and multivalent glycoconjugate vaccines are available for NmA, -C, -W and -Y and their application has provided most promising results.16

Though safe and effective, glycoconjugate vaccines are under debate because of high production costs that may limit broad application in afflicted regions.17 Up until today, the production starts with mass fermentation of pathogens, a biohazardous step that requests the high-tech infrastructure of modern industrial plants10 and limits the build-up of the production infrastructure in indigent regions like the countries of the African sub-Saharan meningitis belt. However, the exigence of decentralised vaccine production has gained conspicuous actuality in the 2015 meningitis season, when an NmC outbreak in Niger could not be stopped because of a shortage in vaccine provision.18

Considering that no licenced NmX vaccine exists today and capitalising on our recent success with exploiting recombinant capsule polymerases (CPs) for in vitro production of bioidentical CPSs,19,20 we focused this study on the production of a synthetic NmX vaccine. With recombinant CsxA, the CP of NmX, we established reaction conditions that yielded the nature identical in vitro produced CPSX (henceforth referred to as CPSXiv to differentiate it from CPSXn, the polymer isolated from natural source) in homogenous quality. In a mouse vaccination experiment, a glycoconjugate vaccine prepared from CPSXiv was found to induce bactericidal antibodies at titres not different form the benchmark.21 The process line exemplified for NmX can be easily adjusted for the production of vaccines against other Nm serogroups and thus should have model character for all glycoconjugate vaccines that start with the biohazardous step of pathogen fermentation.

Results

In vitro synthesis of oligosaccharide primers

Recently we described the small scale production of CPSXiv by use of recombinant CsxA.19 Besides the chemically pure donor sugar UDP-N-acetylglucosamine (UDP-GlcNAc), short priming oligosaccharides (primCPSX) were needed to maximise the reaction efficacy and were obtained through hydrolysis of CPSXn.19 As it was our aim to avoid the use of Neisseria-derived materials to the greatest possible extent in the current upscaled reactions, we first produced primCPSXiv (Figure 1a). Still starting with primCPSXn, three consecutive CsxA catalysed reactions (reactions 1–3) were carried out. Priming oligosaccharides in reactions 2 and 3 were derived from purified and hydrolysed CPSXiv produced in reactions 1 and 2, respectively. In reactions 1–3, priming oligosaccharides were mixed with a 1,000-fold molar excess of UDP-GlcNAc, resulting in a >109 fold dilution of the initially used primCPSXn. Because acidic hydrolysis cleaves the phosphodiester bond in CPSX proximal to the anomeric C-atom (Figure 1b), oligosaccharides obtained from reaction 3 were enzymatically treated to release the phosphate group from the non-reducing end and thus maximise the concentration of functional primers. Anion-exchange chromatography (AEC) used to purify this final primCPSXiv pool as well as high-performance anion-exchange chromatography with pulsed amperometric detection (HPAEC-PAD; Figure 1a) identified fragments ranging in size between DP1–DP8 (DP, degree of polymerisation), for which an average DP (avDP) of 4.5 was calculated based on 1H NMR analysis.21

Figure 1
figure 1

The priming oligosaccharide fraction and evaluation of reaction conditions. (a) HPAEC-PAD profiling shows that the primCPSXiv pool used for upscaling the CPSXiv synthesis contains the (oligo)saccharide species DP1–DP8. The minor peaks preceeding DP3–DP8 indicate the presence of small amounts of oligomers with non-reducing end phosphate groups. (b) Chemical structure of CPSX. Pde, phosphodiester; red. end, reducing end. (c) To determine the D/A ratio that allows complete consumption of UDP-GlcNAc, CsxA reactions were carried out with a constant donor (10 mM UDP-GlcNAc) and varying acceptor (primCPSXiv) concentrations to give D/A ratios as indicated. After overnight incubation, the product spectra were analysed by HPLC-AEC. Although a small peak indicating residual UDP-GlcNAc was visible at the D/A ratio 950, conversion to UMP was complete at D/A ratio 460. CPSX, NmX capsule polysaccharide; CPSXiv, in vitro produced CPSX; HPAEC-PAD, high-performance anion-exchange chromatography with pulsed amperometric detection; HPLC-AEC, high-performance liquid chromatography based anion exchange chromatography.

Determination of efficient reaction conditions

Because the donor-substrate UDP-GlcNAc (henceforth referred to as donor, D) is the single reaction component of appreciable economic value, completeness of conversion into CPSXiv is a critical aspect. With the primCPSXiv fraction of avDP4.5 (henceforth referred to as acceptor, A) at hand, a titration experiment was carried out to determine the D/A ratio that allowed complete consumption of UDP-GlcNAc. The donor concentration was kept at 10 mM and the acceptor increased to give D/A ratios between 4,600 and 90 (Figure 1c). The reactions were run overnight and products separated and visualised using our recently developed high-performance liquid chromatography based anion exchange chromatography (HPLC-AEC) assay.20 Complete conversion of UDP-GlcNAc to UMP was seen at a D/A ratio of 460. However, because the basis of the product peak, an indicator of product dispersity, had considerably broadened from D/A ratio of 950 to D/A ratio of 460, we decided for the D/A ratio of 800 to set-up medium-scale CPSXiv productions.

Scaling up CPSXiv production and product characterisation

The first upscaled reaction was calculated to give 35 mg CPSXiv. As before, UDP-GlcNAc consumption and product synthesis were visualised by HPLC-AEC (shown for start and end point in Figure 2a). After overnight incubation all UDP-GlcNAc was converted to UMP with the corresponding CPSXiv peak detected at 214 nm. A close to 100% reaction yield was confirmed when the mixture was analysed by 31P NMR (Figure 2b). Two main peaks representing UMP and Pde (phosphodiester bonds) appeared and integration of peak areas resulted in a 1:1 ratio. With only trace amounts of GlcNAc-1P, a product of a hydrolytic side activity of CsxA,19 the highly sensitive 31P NMR analysis corroborated the chosen reaction conditions. To control reproducibility, a second reaction was calculated to give 112 mg and was carried out in triplicate. The analytical HPLC-AEC profiles obtained for these reactions clearly confirmed the reliability of the CPSXiv production procedure (Supplementary Figure 1).

Figure 2
figure 2

Synthesis and physico-chemical characterisation of CPSXiv. (a) Completeness of the reaction scaled to give 35 mg CPSXiv was monitored by HPLC-AEC. After overnight incubation, the donor (UDP-GlcNAc) peak was replaced by a UMP peak and the corresponding CPSXiv peak was recorded at 214 nm. (b) 31P NMR analysis of the reaction mixture identified two major peaks representing UMP and Pde. Peak area integration gave equal numbers, thus confirming the quantitative integration of the donor into CPSXiv. The signal for the side product GlcNAc-1P did not exceed trace concentration. (c) 1H NMR used to control purification results and chemical identity between CPSXiv and CPSXn confirmed both, homogeneity and bio-identity of the CPSXiv fraction. CPSX, NmX capsule polysaccharide; CPSXiv, in vitro produced CPSX; CPSXn, CPSX obtained from natural source; HPLC-AEC, high-performance liquid chromatography based anion exchange chromatography; p.p.m., parts per million.

Because the CPSXiv production was started with ultrapure reagents and yielded close to 100% donor consumption, the product purification steps were limited to salt removal by dialysis and AEC to separate CPSXiv from UMP and GlcNAc-1P traces (data not shown). Product purity and identity were confirmed by 1H NMR (Figure 2c). If compared with the crude reaction mixture (bottom panel), it is immediately obvious that the two-step purification procedure delivered homogenously pure CPSXiv (middle panel). Moreover, co-analysis of CPSXn (top panel) demonstrated chemical identity of the two polymers. As a final step, we compared the size of CPSXiv and CPSXn chains using HPLC size exclusion chromatography. With a relative molecular mass of 308 kDa, CPSXiv perfectly mimicked the natural product CPSXn with a relative molecular mass of 388 kDa (Supplementary Figure 2a).

Preparation of a CPSXiv-based glycoconjugate vaccine

For the preparation of a CPSXiv-based vaccine we precisely followed the protocol previously established for CPSXn.21 First, 120 mg of the synthetic polymer were hydrolysed to shorten the CPS chains and the reaction was monitored by 31P NMR.22 Hydrolysis was stopped after 270 min when 31P NMR analysis roughly indicated an avDP12 (Supplementary Figure 2b). The mixture was loaded onto an AEC column to remove oligosaccharides shorter than five to six repeating units. Two pools containing different oligosaccharide polydispersions were collected (Supplementary Figure 2c). Pool 2 contained 84.7 mg of oligosaccharides (70% recovery), which, as identified in an analytical HPAEC-PAD run, exhibited an overlapping dispersity with the benchmark CPSXn of avDP15 (Supplementary Figure 2d). However, with avDP10 (calculated based on 31P NMR analysis; see Supplementary Figure 1d), pool 2 slightly deviated from the benchmark (avDP15). Finally, the perfect congruence of the 1H NMR spectra obtained for the oligosaccharide fractions prepared from CPSXiv and CPSXn confirmed their chemical identity (Figure 3a).

Figure 3
figure 3

Generation of a CPSXiv-based glycoconjugate. (a) To ensure matching of the oligosaccharide fraction generated from CPSXiv and CPSXn, 1H NMR spectra were recorded and showed perfect correspondence. (b) Schematic representation of CPSX hydrolysis and coupling of the resulting oligosaccharides to the protein carrier CRM197. The reducing end sugars are marked in red. (c) The efficacy of oligosaccharide coupling to CRM197 was controlled by HPLC size exclusion chromatography with detection of the conjugates via absorption at 214 nm. Similar to the benchmark (CPSXn-CRM197), CPSXiv-CRM197 elutes in two major peaks. In line with the lower avDP of CPSXiv oligosaccharides (avDP10, Pool 2), the second peak showed a mild shift to lower molecular masses. Importantly, no free CRM197 was detected. CPSX, NmX capsule polysaccharide; CPSXiv, in vitro produced CPSX; CPSXn, CPSX obtained from natural source; HPLC, high-performance liquid chromatography; p.p.m., parts per million.

Conjugation of CPSXiv fragments to the protein carrier CRM197, a non-toxic variant of the diphtheria toxin,23 followed the coupling technology successfully used by Micoli et al.21 to produce the CPSXn-based vaccine MenX-ADH-SIDEA-CRM197 (referred to as CPSXn-CRM197).21 As schematically illustrated in (Figure 3b), coupling to CRM197 proceeds via the reducing end of the oligosaccharides (marked by red squares). Successful coupling was confirmed by HPLC size exclusion chromatography. Similar to our benchmark, CPSXn-CRM197, the new glycoconjugate CPSXiv-CRM197 showed a bipartite elution profile in the absence of detectable amounts of free CRM197 (Figure 3c). However, in line with the smaller size of the oligomer fraction, the second peak was shifted right. CPSXiv-CRM197 was then purified by hydrophobic interaction chromatography and, as a final step in the quality control process, established protocols21,24 were used to determine oligosaccharide loading of CRM197 and control for the presence of free saccharide. These control experiments were done in parallel with CPSXn-CRM197 (Table 1).

Table 1 Comparative characterisation of CPSXiv-CRM197 and CPSXn-CRM197

Immunogenicity testing in mice

The ability of CPSXiv-CRM197 to elicit protective antibodies was tested in a mouse model in comparison with CPSXn-CRM197.21 Figure 4a illustrates the immunisation scheme. After the collection of pre-immune sera at day 0, female BALB/c mice (eight animals per group) were subcutaneously injected with the first dose (day 1; 1 μg saccharide content per dose, formulated in phosphate-buffered saline buffer, pH 7.2, with aluminum phosphate as adjuvant). The injections were repeated twice at day 14 and day 28. Post immunisation, sera (post) were taken at day 27 (Post 2) and day 42 (Post 3). Control animals were treated in the same scheme with phosphate-buffered saline plus adjuvant. Immunoglobulin G (IgG) titres induced were detected using our recently developed ELISA (enzyme-linked immunosorbent assay).21 Comparable IgG titres obtained with the two glycoconjugate vaccines indicate identical immunological properties for CPSXiv-CRM197 and CPSXn-CRM197 (Figure 4b). Moreover, it is of note that considerable IgG titres had established already after two injections (Post 2 sera) and only increased by factor 2–3 after the third vaccine application (CPSXn-CRM197: P=0.028, CPSXiv-CRM197: P=0.0284; Mann–Whitney test).

Figure 4
figure 4

Immunogenicity of CPSXiv-CRM197 in comparison with CPSXn-CRM197. (a) Vaccination schedule showing the immunisation and bleeding of mice. (b) The anti-CPSX IgG ELISA used to determine immunisation results demonstrated comparable IgG responses to CPSX with both, the synthetic (CPSXiv-CRM197) and the benchmark (CPSXn-CRM197) vaccine. Each symbol represents an individual animal. The horizontal bars indicate the geometric mean titre and 95% confidence intervals. *Significant differences between the indicated groups with P<0.05 (CPSXn-CRM197: P=0.028, CPSXiv-CRM197: P=0.0284; Mann-Whitney test). CPSX, NmX capsule polysaccharide; CPSXiv, in vitro produced CPSX; CPSXn, CPSX obtained from natural source; IgG, immunoglobulin G.

Eventually we measured bactericidal activity against NmX strain Z9615. Here, sera isolated from each group and time point were pooled and rabbit serum was used as complement source.21 Comparable bactericidal activity (one dilution step is within the variation of the assay) measured in sera collected from CPSXiv-CRM197 and CPSXn-CRM197 immunised mice convincingly evidenced the value of the described alternative and biohazard-free protocol for the production of an NmX vaccine (Table 2).

Table 2 Rabbit serum bactericidal activity assay

Discussion

For the first time, we describe in this study the use of in vitro synthesised nature identical CPSXiv for the production of a synthetic NmX glycoconjugate vaccine candidate (CPSXiv-CRM197). In a mouse immunisation study, CPSXiv-CRM197 competed with the benchmark vaccine CPSXn-CRM197 (ref. 21) in terms of immunogenicity and elicitation of bactericidal antibodies. We chose NmX to pioneer the enzyme-catalysed vaccine production process, because this serogroup has gained prevalence worldwide17,2531 and outbreaks in Niger,25 Uganda and Kenya,31 and in Togo and Burkina Faso17,30 have forcefully evidenced the need for a specific vaccine. Moreover, in the absence of a licensed NmX vaccine, the implementation of an alternative production scheme should be expedited.

As highlighted by the Global Alliance for Vaccines and Immunisation, a key determinant towards improved health and economic conditions in low-income countries is their access to vaccines (vaccines against poverty).3234 The production process described in this study should be a quantum leap in this regard. Starting from well-defined and pyrogen-free chemicals (UDP-GlcNAc and primCPSXiv) and completely excluding biohazards, the process provides a vantage ground for the build-up of the production infrastructure in indigent regions and thus increase their flexibility to reply to unforeseen needs.18 In addition, stockpiling of vaccines and of vaccine components (for example, oligosaccharide fractions ready for coupling) as requested by the International Coordinating Group on Vaccine Provision for Epidemic Meningitis would be facilitated with the new technology. Of utmost importance in this context is that analytical steps to guarantee safety, homogeneity and lot consistency are facilitated in the fermentation-free procedure.35

The described conditions allowed close to 100% conversion of the donor sugar into polymer. Small oligosaccharides that accrue in hydrolysis and sizing steps provide the optimal starters for new production rounds and a simple HPLC-based analysis enabled on-line process control. Last, but certainly not the least, the recombinant CsxA can be produced in high quality. Without any further optimisation, the enzyme purified from only 1 litre of non-pathogenic E. coli M15(pREP4) culture (OD600=3.0; ref. 19) would have sufficed to generate 8 g CPSXiv. This value is remarkable, given the fact that yields of homogenously pure CPSXn (isolated from fermented bacteria) range between 10 and 600 mg/l.21,3639 Nevertheless, significant room remains for further process optimisation, in particular at the level of the recombinant enzyme. First, solid phase coupling and reuse of the enzyme in repeated production rounds would simplify and enhance the process. Second, the capsule polymerase per se can be engineered towards enhanced yield, solubility and/or stability,20,40 to acquire process-adjusted elongation modes,41 and, eventually, increased flexibility towards chemically functionalised acceptors. The latter could help reducing the coupling chemistry.20

A difference detected between the tested vaccines was a variation in the oligosaccharide dispersion (avDP10 in CPSXiv-CRM197 versus avDP15 in CPSXn-CRM197), a feature most likely attributable to the smaller scale of the CPSXiv hydrolysis reaction. Although more studies are needed to finally decide if this difference is of relevance, the fact that immunisation results did not reflect any associated variance suggests that it is negligible.

In contrast to CPSX, which represents a simple homopolymer of GlcNAc-1P repeating units, CPSs from other Nm serogroups are more complex and in vitro production would need more than one enzymatic activity. We could recently demonstrate on an analytical scale that the herein-presented technology can potentially be expanded to more complex biosynthesis systems. The acetylated CPS of NmA could be produced in a one-pot reaction using three different recombinant enzymes,20 we have done pioneering steps towards the fermentation-free production of the dimeric CPSs of NmW and Y42,43 and, as an example for the most complex CPS expressed by Nm, we also described the synthesis of the trimeric CPS of NmL.44

Taken together, this paradigmatic evaluation of a biohazard-free protocol for the production of an efficient NmX vaccine should pave the way for future decentralised glycoconjugate vaccine production and thus back up the mission for vaccines against poverty.32

Materials and Methods

Synthesis and purification of primCPSXiv

CPSXiv was synthesised in vitro using the recombinant capsule polymerase CsxA expressed as MBP-CsxA-His6 fusion construct.19 Hydrolysis of 0.5 mg CPSXiv (2.5 mg/ml) was performed in 50 mM sodium acetate buffer at pH 4.0 and 80 °C for 6 h. NaOH was added to readjust pH 7 before the mixture was dialysed against water (ZelluTrans, Roth, 1 kDa MWCO) and freeze-dried. Alternatively, primCPSXiv were recycled from pool 1 containing oligosaccharides <DP10 (see Supplementary Figure 1c). For the dephosphorylation of oligosaccharides, we used either acid phosphatase (Worthington Biochemical Corporation, Lakewood, NJ, USA) or calf intestinal alkaline phosphatase (CIP, NEB) and followed the manufacturer’s guidelines. Although removal of acid phosphatase from primCPSXiv was achieved with Amicon centrifugal devices (10 MWCO), CIP was removed by AEC. Individual oligosaccharides were separated on an ÄKTA-FPLC (GE Healthcare, Little Chalfont, Buckinghamshire, UK) equipped with a MonoQ HR 5/5 column (GE Healthcare) at a flow-rate of 1 ml/min. H2O and 1 M NaCl were used as mobile phases M1 and M2, respectively. The samples were separated using a combination of linear gradients (0 to 5% M2 over 1 ml, 5 to 20% M2 over 10 ml, 20 to 30% M2 over 20 ml). Saccharide-containing fractions were pooled and desalted by dialysis (ZelluTrans, Roth, 1 kDa MWCO) against a 1,000-fold excess of water. Fractions containing DP3, DP4 and DP5 were isolated and the DP was confirmed by 1H NMR and HPAEC-PAD as described in refs 21,22.

Upscaling of the in vitro CPSX synthesis

Test reactions in 25 μl of total reaction volume were performed as described before19 in the presence of varying amounts of primCPSXiv to determine conditions suitable for the production of long CPSX chains and complete consumption of UDP-GlcNAc. The analysis of the reaction products by HPLC-AEC was performed following established protocols.19,20,44 For upscaling, 80 mg of UDP-GlcNAc were incubated with 0.6 or 2.5 nmol (62.5 or 250 μg, for overnight or 4 h reactions, respectively) MBP-CsxA-His6 at 37 °C in the presence of primCPSXiv in a total volume of 12.4 ml allowing the synthesis of a maximum of 35 mg CPSXiv. The synthesis of 112 mg CPSX was upscaled accordingly. UMP and other reaction constituents were removed by Tangential Flow Filtration using Vivaflow 50 membranes with 30 kDa MWCO. Alternatively, the reaction volume was reduced to 5 ml by freeze-drying and applied to an ÄKTA-FPLC (GE Healthcare) equipped with a MonoQ 10/100 GL column (GE Healthcare) at a flow-rate of 5 ml/min. H2O and 1 M NaCl were used as mobile phases M1 and M2, respectively. The separation was performed using a combination of linear gradients from 0 to 15% M2 over 24 ml and from 15 to 100% M2 over 224 ml. CPSX-containing fractions were pooled, dialysed against H2O and freeze-dried. Acidic hydrolysis was performed for 4.5 h as described above and the avDP was estimated by 31P NMR.22 The hydrolysate was loaded onto a Q Sepharose column (GE Healthcare) equilibrated with binding buffer (5 mM sodium acetate, pH 7.0). Small oligosaccharides (<DP5-6) were removed with binding buffer containing 200 mM NaCl (pool I; Supplementary Figure 1c) and longer oligosaccharides were eluted with binding buffer containing 1 M NaCl.

Generation and immunogenicity of CPSXn-CRM197

Immunisation protocol, serum analysis, ELISA and rSBA

All methods concerning the generation and characterisation of CPSXiv-CRM197 as well as the immunisation protocol and serum analysis were performed as described before.21 NmX strain Z9615 was kindly provided by Gerd Pluschke, Swiss Tropical and Public Health Institute, Molecular Immunology, Basel, Switzerland. The animal studies were performed in accordance with the Italian law, approved by the local Animal Ethics Committee, and authorised by the Italian Ministry of Health.