Assessing general states of the guinea pigs after vaccination
The effect of the vaccine on guinea pigs was evaluated with different ways of administering, with different doses and frequencies of the use of vaccine in comparison with a negative (PBS) control group.
It was found that the vaccine was safe in guinea pigs in different ways of vaccine administering – conjunctival, intranasal and sublingual, as well as in various doses in primary and secondary immunization (prime and boost). There were no animal deaths or signs of disease by the end of the observation period. In general, the condition of the animals, both in the control and in the experimental groups, was satisfactory in terms of physical activity, appetite and general health condition.
Evaluation of changes in animal body weight within 21 days after prime-boost immunization showed that the weight of animals (on average) increased in all test groups (Figure 2) by 45 — 58% and amounted to 158–175 g which was comparable to the control group — 55 % and 162 g.
No group was differed significantly in mean of animal weight from the negative (PBS) control group.
Protectiveness of viral vector based on vaccine candidate at different ways of its administration against B. melitensis 16M infection
The protective efficacy of the vaccine candidate was evaluated in guinea pigs using conjunctival (c.), intranasal (i.n.) and sublingual (s.l.) routes of administration and compared with reference B. melitensis Rev.1 vaccine or PBS control groups.
The protective efficacy of the vaccine was assessed by parameters as the index of infection, the efficacy of vaccination and the number of bacteria of the virulent strain of B. melitensis 16M obtained from organs and tissues of vaccinated and unvaccinated animals.
The results of the bacteriological study showed that with various mucosal routs of immunization, the new anti-brucellosis vaccine candidate provided protection at a level of 1.64 to 2.30 log10 units. In comparison with the unvaccinated control group (PBS), all vaccine samples, regardless of the route of administration, ensured protection of guinea pigs from B. melitensis 16M infection (α=0.0001 – 0.02) (Table 1) .
Table 1 Degree of protective efficacy of the vaccines by different routes of administration in guinea pigs
Vaccine
|
Route of administration
|
Log10 CFU/animal a (mean ± SE)
|
Log10 protection b
|
Value (P) c
|
Influenza viral vector based brucellosis vaccine candidate
|
c.
|
0.56 ± 0.22
|
2.3
|
< 0.003
|
i.n.
|
0.06 ± 0.04
|
2.8
|
< 0.0001
|
s.l.
|
1.22 ± 0.29
|
1.64
|
< 0.02
|
Commercial vaccine
B. melitensis Rev.1
|
s.c.
|
0.48 ± 0.18
|
2.38
|
<0.0005
|
Control (PBS)
|
i.n.
|
2.86 ± 0.19
|
0.00
|
-
|
a Degree of protective efficacy of the vaccines was evaluated by the isolation rate of Brucella from organs and tissues of guinea pigs challenged with the virulent strain of B. melitensis 16M infection. b Log10 protection units were obtained by subtracting the mean log10 CFU of the control (PBS) group from the mean of log10 CFU for the experimental group.
c Compared with control group (PBS).
CFU colony forming units, PBS phosphate-buffered saline, c. conjunctivally, i.n. intranasally, s.l. sublingually.
Protective efficacy of vaccines as evaluated by the isolation rate of Brucella from the tissues of control and experimental groups of guinea pigs on day 30 after challenging with the virulent strain of B. melitensis 16М. Animals were vaccinated with the vector vaccine by prime-boost c., i.n., s.l. at interval of 21 days, and with B. melitensis Rev.1 by single s.c. vaccination. Guinea pigs in negative control group were injected with PBS. The challenge of animals was performed with B. melitensis 16M at a dose of 1.3 log10 CFU/animal using s.c. route.Statistical analysis was performed using two-way ANOVA followed by Tukey’s multiple comparisons test.
Significant protection of the vaccine was observed after i.n. administration (2.8 log10), whereas for s.l. immunization, the unit of protection was 1.64 log10. In case when the vaccine administered by c. route the unit of its protection was 2.3 log10, which was comparable to the commercial B. melitensis Rev.1 vaccine results.
According to the index of infection (Figure 3, B), significant protection compared to the control group (PBS) was achieved in the groups vaccinated c. (P < 0.01; vaccination efficiency 60%) and i.n. (P < 0.002, vaccination efficiency 80%), as well as in animals vaccinated with B. melitensis Rev.1 (P < 0.005; vaccination efficiency 80%). It should be noted that the index of infection in i.n. vaccinated animals was similar (P > 0.99) to the index in animals immunized with the commercial B. melitensis Rev.1 vaccine.
Based on the results of these studies, the i.n. route of vaccine administration was applied for further research in order to determine the optimal dose for immunization.
Study of protective efficacy of a novel vaccine candidate at different doses and after infection with B. melitensis
In this study, the protectiveness of the vaccine was assessed at various doses of i.n. vaccine administration after prime-boost immunization, as well as after challenge of guinea pigs with the virulent B. melitensis 16M strain.
The evaluation of the protective efficacy of the tetravalent vector brucellosis vaccine against the infection was carried out according to the following parameters — 1) determination of the effectiveness of vaccination (the degree of complete protection against infection, expressed in percent), 2) study of the infection index, as well as by counting Brucella colonies in the tissues and lymph nodes of guinea pigs 30 days after infection.
Bacteriological studies of the organs and lymph nodes of infected animals showed that the tested doses of the recombinant vector vaccine, as well as the commercial vaccine, provided significant protection (P < 0.04 versus the unvaccinated group) of guinea pigs against B. melitensis 16M infection ranging from 1.64 to 2.8 log10 units. Our results showed that the highest level of protection (vaccination efficiency) against infection in guinea pigs was in the groups immunized at doses of 106 EID50 and 107 EID50 (80%) compared with the control group (PBS) after the challenge, in which the infection rate was 100% and these data were statistically significant (P < 0.04). It should be noted that in the group vaccinated with B. melitensis Rev.1 the vaccination efficiency was also 80% (Table 2).
According to the index of infection (Figure 4, D), a significant level of protection in comparison with the control group (level of infection: 100%) was achieved in all three tested doses and only after secondary boost vaccination (P < 0.0004, P < 0.02). The index of infection in the groups of animals immunized with a dose of vaccine 106 EID50 and B. melitensis Rev.1 vaccine was comparable with each other and these groups differed significantly compared to the negative control group P = 0.003–0.001.
Table 2 Rates of protection in guinea pigs after challenge with the virulent strain B. melitensis 16M
Immunization group (prime-boost)
|
Total animals
|
Isolation of B. melitensis in animals, n (%)
|
Value (P) a
|
(+) control b
|
(-) control c
|
Vector vaccine at dose of 105 EID50
|
5
|
2 (40)
|
> 0.05
|
> 0.05
|
Vector vaccine at dose of 106 EID50
|
5
|
1 (20)
|
> 0.05
|
< 0.05
|
Vector vaccine at dose of 107 EID50
|
5
|
1 (20)
|
> 0.05
|
< 0.05
|
B. melitensis Rev.1
|
5
|
1 (20)
|
-
|
< 0.05
|
Control (PBS)
|
5
|
5 (100)
|
< 0.05
|
-
|
a in comparison with control untreated PBS or B. melitensis Rev.1 groups. b animals immunized with B. melitensis Rev.1 vaccine. c animals inoculated with PBS. EID50 50 percent embryo infectious dose.
Guinea pigs were immunized twice intranasally 21 days apart with a new vaccine candidate at dose 105 EID50, 106 EID50 and 107 EID50 or a single delivery of the vaccine B. melitensis Rev.1. via s.c. immunization. Animals challenged with virulent strain of B. melitensis 16M at a dose of 1.3 log10 CFU/animal using subcutaneous route. Statistical analysis was performed using a one-sided Fisher’s exact test. P-value less than 0.05 (< 0.05), P-value higher than 0.05 (> 0.05).
It should be noted that the values of the index of infection between the B. melitensis Rev.1 group and the experimental groups did not have significance (P > 0.05).