Immunogenicity and protective efficacy of a live, oral cholera vaccine formulation stored outside-the-cold-chain for 140 days

Cholera, an acute watery diarrhoeal disease caused by the waterborne bacterium Vibrio cholerae is endemic and epidemic in 69 low-and middle-income countries (LMICs) [1‐3]. It is predominantly caused by V. cholerae serogroups O1 El Tor, and in Asian countries, mostly by O139 [4‐6] and the evolution of new toxigenic strains remains an important global health challenge [7‐9]. The clinical manifestations of cholera caused by V. cholerae O1 versus O139 are indistinguishable. Vaccination is a preventive measure and killed oral cholera vaccines for O1 and O139 and a live vaccine for O1 are available. Markedly, the vaccine for O1 does not cross-protect against cholera caused by O139 and vice versa [10‐14]. Killed vaccines confer short-term protection and require a booster dose as opposed to a single-dose live attenuated vaccine that mimics natural infection and eliminates repetitive dosing [15‐18]. Although all the existing WHO licensed cholera vaccines are safe, they demand a cold chain supply (2–8 °C) distribution system from manufacturing to the immunization site to ensure their safety and potency and cold chain logistics are difficult to execute in LMICs [19, 20]. Hence, these mandatory requirements resulted in a high cost of vaccination which poses a great challenge [21, 22]. A cold chain free version of any cholera vaccine would relieve the bottlenecks and cost determinants and result in significant cost savings during mass vaccination campaigns [23‐25]. Therefore, it is inevitable to develop a single dose and cold chain free live cholera vaccine.

Live cholera vaccine candidates have been developed by attenuation of virulence in the pathogenic strains by genetic engineering. However, in the development of a live attenuated cholera vaccine candidate, the degree of attenuation has been hampered by its unacceptable clinical side effects or reactogenicity (adverse reactions) in volunteers, such as a headache, vomiting, diarrhoea, including noncholeric diarrhoea and abdominal cramps, which are a cause of concern when compared to the vaccines formulated with heat-killed cells [26, 27]. Hence, the vaccine candidate must be genetically stable, immunogenic and unable to revert to the pathogenic phenotype. Towards this, several live attenuated vaccines against O1 and O139 are in various stages of development and evaluation with the vaccine candidates CVD-103 HgR [28, 29], VA1.3/VA1.4 [30], Peru-15 [31], IEM 101/108/109 [32], Cuban 638 [33, 34], Texas Star [35] and Wzm [36], CVD112 [37], Bengal-15 [38], TLP01 [39], VRI-16 [40] and L911/L912 [41]. However, similar to killed cholera vaccines, live vaccine formulations are also heat-sensitive and cold chain supply dependent. Therefore, a cold chain-free, live, attenuated cholera vaccine that can be stored at room temperature must be developed to increase its outreach to global immunization programmes.

Notably, there is no live vaccine exclusively available to protect against cholera caused by V. cholerae O139 and to date, no cold chain-free live attenuated oral cholera vaccine against O1 and O139 has been commercialized. In this direction, live attenuated aminolevulinic acid (ALA) auxotroph VCUSM1 and VCUSM2 strains protective against V. cholerae O139 were constructed by frameshift mutation of a housekeeping gene, hemA that encodes for glutamyl-tRNA reductase, an important enzyme in the C5 pathway for delta-aminolevulinic acid (ALA) biosynthesis, which renders this strain dependent on exogenous ALA for survival and these vaccine candidates were patented [42, 43]. The VCUSM2 was found to be immunogenic but showed mild reactogenic effects in animal models due to the presence of two copies of cholera toxin genetic element. Hence, this strain was further improved by mutating the ctxA gene via substitution of 7th amino acid, arginine to lysine, R7K, and 112th amino acid, glutamate to glutamine, E112Q. And, two copies of ace and zot genes in ctx operon were also deleted to reduce the reactogenicity and resultant strain VCUSM14 (an aminolevulinic acid (ALA) auxotrophic and non-reactogenic) was characterised and evaluated in animal models [44]. Further, the hemA gene was reintroduced into VCUSM14 to enhance its colonization potential, and the strain was designated as VCUSM14P. The VCUSM14P is a non-toxigenic strain and an aminolevulinic acid (ALA) prototroph with enhanced colonization and immunogenic properties against infection by the V. cholerae O139 serogroup.

The development of cold chain free, live liquid vaccine formulation was based on the understanding of the survival mechanisms of both toxigenic and nontoxigenic V. cholerae strains that inhabit nutrient-poor, temperature and oxygen fluctuating levels in aquatic ecosystems year-round. These adaptive traits of V. cholerae were leveraged at an in-vitro condition that best mimic the environmental stress conditions for the extended storage period of live attenuated cholera vaccine strain VCUSM14P at room temperature (25 °C ± 2 °C). Eventually, a prototype cold chain-free, live-attenuated oral cholera vaccine (LACV) formulation with VCUSM14P was developed and a ‘Patent Filed’. The LACV is a liquid formulation consisting of 5 × 10⁶ CFU/mL of the VCUSM14P strain. Accelerated storage stability studies were performed for six batches of LACV in an ICH-compliant stability chamber (Binder-KBF 115, Germany) at 25 °C ± 2 °C and 60% ± 5% relative humidity (RH). At fixed intervals, the viability of the VCUSM14P strain in the LACV was enumerated and its genetic purity was ascertained by polymerase chain reaction. The statistical analysis was performed by using the Wilcoxon Rank Sum Test and no significant differences observed between the batches. The LACV was found stable at 25 °C ± 2 °C and 60% ± 5% RH by retaining its viability, purity and potency for 140 days. After 140 days, the cell viability was decreased by one to two orders of magnitude and hence the LACV was not tested further for its safety and efficacy. The repeated dose toxicity of the LACV was evaluated in Sprague Dawley (SD) rats to ascertain its safety for clinical use [45]. The present study focused on the evaluation of colonization potential, reactogenicity, immunogenicity and protective efficacy of the LACV after its storage at room temperature for 140 days in animal models for the development of a single-dose, cold chain-free, live oral cholera vaccine against V. cholerae O139.

A single-dose cold chain-free cholera vaccine would cost less due to its storage and distribution at room temperature. An ideal live attenuated oral cholera vaccine should colonize effectively, be non-reactogenic and immunogenic and induce a protective immune response against a challenge. Therefore, this study focused on the evaluation of a LACV for these key attributes. Intestinal colonization is a pre-requisite for the establishment of infection and subsequent elicitation of the immune response [46‐48]. It was proposed that an inoculum containing V. cholerae 10³–10⁸ cells is required for an effective infection of a human host [49]. In agreement with this hypothesis, in the present study, we found an increased colonization potential of the LACV at a dose of 2.5 × 10⁵ CFU/50 μL in infant mice. Similar to our results, a dose of 10⁵ CFU of V. cholerae (El Tor strain C6706) was effective in colonization and biofilm development in infant mice, as reported in [50]. In contrast, the VCUSM2, VCUSM14 and VCUSM21P strains were recovered with 1.8 × 10⁵ CFU, 2.0 × 10⁴ CFU and 1.55 × 10⁶ CFU respectively, from mouse intestines [44, 51]. In comparison to the recovery of these VCUSM strains, a two-log higher recovery of VCUSM14P was recorded in the present study. The higher colonization potential of the LACV could be due to the mutation in ctxA, deletion of the ace and zot genes and the presence of the hemA gene in the vaccine (VCUSM14P) strain.

The safety of a live attenuated cholera vaccine is mainly focused on its reactogenicity. Reactogenicity (adverse reactions) of a live attenuated cholera vaccine in volunteers is a cause of concern [52] and dependent on V. cholerae flagellins [27]. Reactogenicity of a cholera vaccine has been assessed based on the fluid accumulation ratio (FAR) in rabbit ligated ileal loops. A FAR greater than 1.0 indicates a strong toxigenicity of cholera toxin and less than 0.2 indicates no reactogenicity [53, 54]. In unvaccinated rabbits, the loops injected with the LACV and unformulated VCUSM14P were recorded with less than a 0.09–0.16 FAR. In contrast, the loops injected with WT O139 exhibited a 4-fold increase in FAR, which correlates with the symptoms of acute cholera. In addition to fluid accumulation, bloody mucus was observed in loops inoculated with the WT O139 strain, indicating haemorrhage. Similar observations were reported with WT O139 infections in a rabbit [55]. Our results indicate that both the LACV and unformulated VCUSM14P had no detectable diarrhoeagenic activity even at an inoculation dose of 10⁴–10⁶ CFU/mL in a rabbit ileal loop model without signs of haemorrhage and reactogenicity. A similar observation with VCUSM14 at doses of 10⁶ and 10⁸ CFU was reported by [44].

A RITARD assay was performed to further validate the results of the rabbit ileal loops assay. Rabbits vaccinated with the LACV formulation or unformulated VCUSM14P survived the challenge with WT O139 and showed no signs of diarrhoea or other symptoms of disease or death for up to 5 days of the observation period. However, unvaccinated rabbits developed cholera symptoms, and 100% mortality was observed in unvaccinated rabbits within 24 h post-challenge. Our RITARD results similar to those of V. cholerae ghost (VCG) vaccine candidate [56] and purified outer membrane vesicle [57] protection against virulent V. cholerae O1 (El Tor) and O139 strains. Similarly, our findings are also in agreement with protection by the live attenuated cholera vaccine VA1.4 against WT O139 in the RITARD model [30].

The excretion of vibrios in a vaccinated rabbit’s faecal material is a marker of intestinal colonization. Prolonged shedding of vibrios indicates successful colonization and subsequent multiplication of the vibrios in the small intestine [58]. Shedding of vibrios by the vaccinated rabbits after the first immunization indicates successful colonization of the vaccine strain, which correlates with our findings in the RITARD study and mouse colonization assay. No shedding of the vaccine strain was recorded after the booster dose. This result illustrates that the immune response induced by the first immunization was efficient enough to eliminate the bacteria used for the second immunization. This observation was supported by the lack of fluid accumulation in vaccinated rabbits, indicating the presence of sufficient anti-CT neutralizing antibodies to prevent fluid accumulation in the intestinal loops.

Several studies have demonstrated the cholera toxin-neutralising ability of anti-CT IgG and IgA antibodies when animals are challenged with live toxigenic V. cholerae [59, 60]. An increase in anti-CT IgG/IgA titres would protect the host from cholera by neutralizing CT [61]. The vibriocidal assay has been an indicator to measure the protective efficacy of a vaccine against cholera [30, 62]. A four-fold or greater increase in serum vibriocidal antibodies is known to confer protective efficacy of a cholera vaccine [47, 52, 63]. In the present study, the pre-immune sera of unvaccinated rabbits were recorded with a low vibriocidal antibody titres (baseline GMT of 10), which indicates that the rabbits were not previously exposed to V. cholerae or related organisms. However, after the booster dose in immunized rabbits, the vibriocidal antibodies were increased by 31-fold with the LACV and 14-fold with unformulated VCUSM14P. The results obtained in this study are comparable to those obtained by [56] in the evaluation of V. cholerae ghost (VCG) vaccine candidates, which induced a 20-fold increase in vibriocidal activity in the vaccinated rabbits. In all of the LACV-vaccinated rabbits, a significant increase in anti-CT IgG and IgA antibody titres from the baseline GMT of 10 to 17.12 and 72.67, respectively, was recorded at the first-week post-vaccination. At 3rd and 4th week, the rabbits elicited increased titres of anti-CT IgG and IgA antibodies. At 4th week, the LACV-vaccinated rabbits exhibited a 275-fold increase in anti-CT IgG and a 15-fold increase in anti-CT IgA antibodies compared to those of the rabbits vaccinated with unformulated VCUSM14P. Similar trends were reported [64] with killed thimerosal-free oral cholera vaccine against V. cholerae O1 Inaba. Overall, our results indicate that both the LACV and unformulated VCUSM14P are capable of inducing the humoral and vibriocidal immune responses against WT O139 and protected vaccinated rabbits, as evidenced by the RITARD results.