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Infection and Immunity, July 2001, p. 4502-4508, Vol. 69, No. 7
Department of Basic and Clinical Immunology,
Finlay Institute, Havana City, Cuba
Received 11 September 2000/Returned for modification 24 October
2000/Accepted 28 March 2001
This report explores the participation of some afferent mechanisms
in the immune response induced by the Cuban anti-meningococcal vaccine
VA-MENGOC-BC. The induction of delayed-type hypersensitivity in nursing
babies and lymphocyte proliferation after immunization is demonstrated.
The presence of gamma interferon IFN- Neisseria meningitidis is
a human pathogen and one of the major causes of bacterial meningitis
(29). Infection may result in the development of
septicemia and/or meningitis, with severe clinical symptoms. Natural
immunity in humans is acquired by meningococcal colonization of the
upper respiratory tract and increases with age (13). In
1969, Goldschneider et al. described an age-related inverse
relationship of the incidence of meningococcal disease and the presence
of bactericidal antibodies (14).
Polysaccharide-based vaccines against some serogroups are available,
but these antigens cannot be used to protect against serogroup B due to
the low immunogenicity of the B polysaccharide in humans
(49); therefore, protein-based vaccines have been developed. VA-MENGOC-BC is the registered trademark of the Cuban vaccine against serogroup B and C N. meningitidis (2,
44). One of the most important findings of the Cuban vaccine
trial was the demonstration, for the first time, that antibodies
induced to noncapsular surface antigens can protect against
meningococcal disease (10). Another important observation
was that VA-MENGOC-BC is innocuous and safe. The vaccine efficacy
surpassed 80% in a double-blind placebo-controlled vaccine trial
conducted in junior high school students (11 to 15 years old)
(24, 44). Yet another finding was the reduction in the
morbidity and mortality rates caused by group B N. meningitidis after its application in all Cuban provinces since
1988 (48). Last but not least was the decreased incidence
in children less than 5 years old from 67 to 120 in 1983 to 0.05 to
0.09 per 105 inhabitants in 1997 (24).
The presence of bactericidal antibodies has been shown to correlate
with natural protection against the disease (14). Such antibodies are observed after infections by serogroup A, C, Y, and
W-135 N. meningitidis and correlate with the protection
induced by their polysaccharide-based vaccines (9, 31,
50). Nevertheless, the presence of bactericidal activity after
immunization with outer membrane vesicle (OMV)-based vaccines such as
VA-MENGOC-BC is controversial (5, 30, 44, 47), but the
induction of such antibodies by noncapsular antigens (9, 10, 38,
39) remains the goal.
The complement-fixing antibodies may have other effector functions and
come from a cellular pattern of immune response. Based on cytokine
production, CD4+ T lymphocytes have been classified as
T-helper 1 (Th1) cells, which produce and favor gamma interferon
(IFN- Our main goal here has been to further our understanding of the
triggering by this vaccine of the afferent and effector branches of the
immune response, considering that serum bactericidal activity is only
one of the multiple mechanisms involved in protection against N. meningitidis B. Particular attention was given to the mechanism
related to Th1 cellular responses. In the afferent branch, DTH, LP, and
production of cytokines at the mRNA level were explored. In the
effector branch, the presence of opsonizing antibodies was
demonstrated, and the role of PMN as effectors was also evaluated.
Vaccine and immunization.
N. meningitidis strain
B:4:P1,19,15 (Cuban vaccine strain) was grown until early stationary
phase, and OMVs were extracted with 0.1 M Tris-HCl [pH 8.6]-10 mM
EDTA-0.5% (wt/vol) deoxycholate. This preparation was purified by
sequential centrifugation steps at 20,000 × g for 30 min. Following ultracentrifugation at 125,000 × g for
2 h, the pelleted OMVs were homogenized in phosphate-buffered saline (PBS; pH 7.2) with 3% (wt/vol) sucrose and further purified by
column chromatography. In addition, the vaccine contains purified capsular polysaccharide of serogroup C meningococcus, both adsorbed on
Al(OH)3 gel (16). The immunization schedule
for humans comprises two doses applied with a 6- to 8-week interval,
whereas for rats there was a 5-week interval. One dose of vaccine (0.5 ml) contained 50 µg of proteins, 50 µg of polysaccharide, and 2 mg
of Al(OH)3 and was administered intramuscularly, deep in
the deltoid muscle in humans and in the posterior extremity of rats.
Immune response induction. (i) DTH response.
A group of 50 healthy nursing babies without history of meningococcal disease were
included in the study after written consent of the parents. They were
immunized twice, at 3.5 months of age and 42 days later. DTH was
measured 28 days after the second dose by multipuncture application of
nonadsorbed OMVs (14 µg) as antigen. The OMV preparation was diluted
(vol/vol) in PBS-glycerol, plus phenol (0.05%); it and the control
(without antigen) were applied in the forearm. Induration areas were
measured 48 h later, and differences greater than 3 mm between
antigen and control were considered positive.
(ii) LP assay.
A group of 20 healthy young adults without
history of meningococcal disease and negative for immunoglobulin G
(IgG)-specific (anti-OMV) antibodies before immunization participated
in this study. They were recruited and included in the study after
written consent. Volunteers were immunized intramuscularly with two
doses of VA-MENGOC-BC at a 6-week interval. Twenty-one days later fresh peripheral blood mononuclear cells (PBMC) were obtained from
heparinized blood by sedimentation on a Ficoll-Hypaque (Pharmacia)
gradient. PBMC were cultured in 96-well round-bottom microtiter plates
(Costar) at a density of 105 cells per well in 200 µl of
RPMI 1640 (Sigma) supplemented with 5% heat-inactivated autologus
serum, 10 µg of gentamicin per ml, and 0.3 mg of
L-glutamine per ml. Nonadsorbed OMVs from strain B:4:P1.19,15 were added at doses of 0.2, 1, 5, and 10 µg per ml. As a
control, PBMC were incubated without the antigen or with phytohemagglutinin (PHA) at a 1% concentration (Gibco). These cells
were incubated for 5 days at 37°C and 5% CO2 (ASSAB,
Sweden) and pulsed with 1 µCi of [3H]thymidine
(Amersham, International Little Chalfont, United Kingdom) over the last
18 h of culture. Cells were harvested, and the incorporated radioactivity was measured in a liquid scintillation counter
(Pharmacia, LKB). Results are expressed as the mean counts per minute
of triplicate cultures. Volunteers with a stimulation index of (iii) Stimulation of cytokine mRNA.
Six adult healthy
volunteers without history of meningococcal disease participated in
this study. They were recruited and included in the study by regular
written consent. They had been immunized with two doses of VA-MENGOC-BC
3 years before. PBMC of each individual were freshly isolated and
cultured individually as described for the LP assay. Two milliliters of
cellular suspension (8 × 106 per well) was incubated with
9.6 µg of OMV antigen (1.2 µg/106 cells); PHA (2 µg/106 cells) and medium were used as controls. The cells
incubated with antigen were harvested after 8, 10, 12, 14, 16, 18, 24, and 72 h of culture. Cells cultured with the mitogen or medium
alone were harvested after 10 h. They were washed three times and
lysed for RNA isolation.
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.7.4502-4508.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Immune Response Induction and New Effector
Mechanisms Possibly Involved in Protection Conferred by the Cuban
Anti-Meningococcal BC Vaccine
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
and interleukin-2 (IL-2) mRNAs
but absence of IL-4, IL-5, and IL-10 mRNAs were observed in peripheral
blood mononuclear cells from immunized subjects after in vitro
challenge with outer membrane vesicles. In addition, some effector
functions were also explored. The presence of opsonic activity was
demonstrated in sera from vaccinees. The role of neutrophils as
essential effector cells was shown. In conclusion, we have shown that,
at least in the Cuban adult population, VA-MENGOC-BC induces mechanisms
with a T-helper 1 pattern in the afferent and effector branches of the
immune response.
INTRODUCTION
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
) and interleukin-2 (IL-2)-mediated cellular immune responses,
and Th2 cells, which produce and favor IL-4-, IL-5-, and IL-10-mediated
humoral responses (25, 35). The cytokine production
associated with T-cell proliferation has also become an important way
to evaluate immune responses. Therefore, the cellular responses
induced by VA-MENGOC-BC, including in vivo and in vitro
responses were evaluated. Delayed-type hypersensitivity (DTH) and
lymphocyte proliferation (LP) have been widely accepted as measures of
T-cell activity. The antibodies that fix complement also have opsonic
activity (36), and the specific immune response is
amplified by the T-helper cascade, which includes intercellular and
cellular responses known as a nonspecific amplification. This means
that the participation of macrophages and neutrophils
(polymorphonuclear leukocytes [PMN]) could be very important in
regulation of the immune response as well as part of the effector
mechanisms against N. meningitidis B infection.
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
2 and
1,000 cpm were considered positive. To avoid exclusion of appropriate antigen-presenting cells, unfractionated PBMC were used in the 5-day
proliferation assay, which is widely accepted as a measure of T-cell activity.
20°C. The pellet was resuspended in 400 µl of solution D and
precipitated again under the same conditions. Finally, the pellet was
resuspended in an adequate volume of diethyl pyrocarbonate-treated H2O (Sigma).
and the L32 and GAPDH (glyceraldehyde phosphate dehydrogenase) housekeeping genes were used
(12). Briefly, using the templates, radiolabeled antisense
RNA probes were synthesized by in vitro transcription reaction using T7
RNA polymerase under appropriate conditions and an excess
[
-32P]UTP (Amersham) (27). The
radiolabeled probes were purified by phenol-chloroform extraction and
ethanol precipitation after the transcription reaction was stopped by
adding 1 µl of RNase-free DNase. Excess purified probes were
hybridized to 5 µg of purified total RNA from samples in
hybridization buffer overnight at 56°C. The free probe and
single-stranded RNA (nonprotected) were digested with RNases A and
T1 in adequate buffer at 37°C for 45 min. The reaction
was stopped by the addition of proteinase K; the remaining RNase-protected probes were purified with phenol-chloroform and ethanol
precipitation, resolved on 5% denaturing polyacrylamide gel, and
autoradiographed. All the reagents and enzymes were provided by the
PharMingen kit. The films were scanned and analyzed using the Molecular
Analyst software (Bio-Rad). Since the undigested radiolabeled RNA probe
contains flanking frames of plasmid DNA, it migrates at lower rates
than protected fragments due to the elimination of nonprotected
flanking frames during RNAse digestion. Because the lengths of probes
and protected fragments for each cytokine are known, a standard curve
was plotted with undigested radiolabeled probes (migration distance
versus log nucleotide lengths) and used to establish the identity of
RNase-protected bands in experimental samples. The quantity of each
mRNA species expression level was determined by the intensity of
appropriately sized protected probes and homogenized using the signal
from an L32 probe used as the standard.
Effector immune mechanisms. (i) Opsonophagocytic activity.
Nine of the volunteers used in the LP assay who had no serum anti-OMV
IgG class antibodies before immunization were included in this study.
Sera were collected before vaccination and 4 weeks after the second
dose. During the second extraction heparinized blood was also obtained
for the purification of phagocytic cells (PMN and macrophages). The
erythrocytes were eliminated with lysing solution, and the leukocytes
resuspended at 1.25 × 107 phagocytic cells per ml in
RPMI 1640 containing 0.5% bovine serum albumin (Sigma). The serogroup
B meningococci (N. meningitidis strain B:4:P1.19,15) were
grown overnight on Mueller-Hinton agar in 5% CO2
atmosphere at 37°C, inoculated in Frantz-modified medium to an
optical density of 620 nm, using a 10-mm light, and grown to
logarithmic phase in an orbital shaker at 37°C. Bacteria were washed
three times in 0.9% NaCl (2,500 × g for 10 min at
4°C), resuspended in RPMI 1640 (pH 7.2), and adjusted to an optical density of 1, and CFU per milliliter was determined. Bacteria were
labeled with fluorescein isothiocyanate (FITC; 0.25 mg/ml) by stirring
the bacteria for 30 min at 37°C in PBS, killed by ethanol (0.1% for
1 h), and filtered through 0.22-µm-pore-size filters
(Sartorious). They were extensively washed in PBS at 2,500 × g for 10 min at 4°C, resuspended in the same medium, counted by flow cytometry, and adjusted to 5 × 108 cells per
ml, and aliquots were stored at 70°C. Bacterial suspensions (5 × 107) were opsonized with 5% autologous sera with or
without active complement (inactivation was performed by treatment for
30 min at 56°C) during 15 min, and the cells were added (1:20,
cell/bacteria) and incubated for 30 min. Phagocytosis was stopped by
adding 1 ml of ice-cold PBS supplemented with 0.02% of EDTA. The
suspensions were analyzed by a Cytofluorograph Ortho 50 H interfaced to
a model 2150 computer (Ortho Diagnostic Instrument, Westwood, Mass.) with a 488-nm wavelength. FITC fluorescence was measured at 515 to 575 nm, and forward angle light scatter was measured at 488 nm.
(ii) PMN as effector cells.
Two assays were performed. In
the first, the in vitro effector activity of PMN against N. meningitidis B (103 bacteria per well) was tested with
human PMN (105 cells per well). The blood was obtained as
described above (100:1, cell/bacteria). The sedimented erythrocytes
were eliminated with lysing solution, and the PMN were resuspended in
RPMI 1640 supplemented with 10% fetal calf serum (Gibco). The cells
were activated with IFN- (10 U/ml) and lipopolysaccharide (LPS; 1 µg/ml) 30 min before addition of the bacteria, and CFU were measured
24 h later. In the second, a rat neutropenic model was used to
determine the role of PMN in vivo. Wistar rats (CENPALAB; Havana, Cuba)
weighing 80 ± 20 g were randomized in three groups of 10 animals each. The first group was treated before challenge with an
unrelated IgM antibody (control), and the second was immunized with 2 doses of VA-MENGOC-BC (25 µg of protein, intramuscularly) 5 weeks
apart; the third group was immunized as was group 2 and 2 h before each dose made neutropenic by intraperitoneal inoculation of 2 ml of ascitic
fluid of an anti-PMN monoclonal antibody (MAb) (RP3, IgM class; kindly donated by F. Sendo, Yamagata University, Yamagata, Japan) (20). MAb efficiency was measured every day in the
peripheral blood by differential counts. All groups were challenged
intraperitoneally with 100 50% lethal doses of N. meningitidis B (strain B:4:P1.19,15). Rat survival was recorded
over 3 days.
Ethical considerations. Since children were included in this work, authorization from the National Group of Paediatrics, health authorities, and the Institutional Ethical Committee were necessary, with prior demonstration of safety and innocuousness. Furthermore, the written consent of each parent or guardian was included.
Statistical analysis. Differences between groups were tested for significance by a paired two-tailed Student's t test. Survival significance was calculated by the exact Fisher probability. The result of RPA analysis was processed with Molecular Analyst software. The X-ray films were digitized using a Hewlett-Packard scanner, and the lengths were determined by comparing the mobility of the bands with that of the undigested probes. The density/area ratios were calculated, and the relative mRNA levels were determined in relation to the density/area ratio of the housekeeping gene L32. The means and standard deviations for the six volunteers were calculated and plotted for each time point measured.
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RESULTS |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Immune response induction. (i) VA-MENGOC-BC induces a DTH
response.
The induction of DTH by VA-MENGOC-BC was evaluated
by measuring DTH before immunization of 3.5-month-old nursing babies
and 30 days after the second dose. Figure
1 shows the effect of this vaccine on the
DTH response. It was negative before immunization, and a remarkable
increase was observed after the second dose in all subjects. Six weeks
after the first dose, DTH was also positive but much less than after
the complete immunization schedule (data not shown).
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(ii) VA-MENGOC-BC induces LP.
LP assays were carried out to
study the T-cell response in vaccinated subjects who were negative for
specific IgG before vaccination started. OMVs from the Cuban strain
B:4:P1.19,15 were used to study the antigen-specific stimulation of
human PBMC 21 days after the second vaccine dose. As shown in Fig.
2, OMVs induced stimulation of PBMC from
young adult humans immunized with VA-MENGOC-BC in a dose-response
fashion.
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(iii) The OMVs of VA-MENGOC-BC induce cytokine mRNA.
The
influence on the cytokine pattern after in vitro OMV challenge of PBMC
from VA-MENGOC-BC immunized adult human subjects was evaluated.
Figure 3A shows the effects of antigenic
stimulation on IFN-, IL-2, and IL-13 mRNAs, which appear to follow
different kinetics. A graphic representation is shown in Fig. 3B.
IFN- and IL-2 relative expression levels began to increase at 8 h, reaching a peak at 14 h of stimulation; a decrease was observed at 16 h. IFN- transcriptional induction increased again up to at least 72 h, when it reached a level similar to that attained at
14 h. IL-2 mRNA induction remained at similar levels after 16 h.
On the other hand, the relative expression of IL-13 showed kinetics
similar to those for IFN-, but at a much lower level. The induction
of IL-4, IL-5, IL-10, IL-14, IL-15, and IL-9 mRNAs were detected in the
PHA controls but not in the samples.
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Effector immune mechanism. (i) Immunization with VA-MENGOC-BC
induces serum opsonic activity.
The influence of antibodies from
VA-MENGOC-BC-immunized subjects (before and 21 days after the second
vaccine dose) and autologous complement as opsonins were studied. As
shown in Fig. 4, opsonic activity
increased after vaccination, and a high percentage of phagocytosed
bacteria were observed in postimmunization specimens. The addition of
autologous complement before or after immunization significantly
increased the opsonizing activity.
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(ii) Neutrophils appear to be essential cells in the defense
against N. meningitidis B.
The killer activity of
human PMN from immunized volunteers was evaluated in vitro and in vivo.
As shown in Fig. 5A, the PMN are
efficient in killing N. meningitidis B whether they are
activated (IFN- plus LPS) or not. In vivo, treatment of rats with
MAb RP3 produces peripheral neutropenia (data not shown) as
reported (20). Figure 5B shows that vaccination
(RP3 group) significantly increases (P < 0.001) survival in rats; in contrast, 100% mortality was observed
in the neutropenic animals after treatment with RP3 at the
moment of challenge with N. meningitidis. Survival in
animals treated with an irrelevant IgM (control) was 30%.
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DISCUSSION |
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Abstract
Introduction
Materials and Methods
Results
Discussion
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VA-MENGOC-BC is a vaccine that was developed two decades ago; nevertheless, not much is known about its fine mechanisms of action. Indeed, the assumption that this OMV-based vaccine necessarily produces its effect only by development of bactericidal antibodies is premature.
The humoral response induced by VA-MENGOC-BC in humans consists of
specific IgG antibody, mainly of IgG subclass (7), with bactericidal activity against some of the most frequent serotype B
N. meningitidis pathogens. Nevertheless, the induction of
bactericidal antibodies, mainly in babies, remains controversial
(2, 30, 47), and no efficacy study has been conducted in
this age group. In our opinion, the induction of bactericidal
antibodies, the hallmark of the polysaccharide-based vaccines and main
goal of the Neisseria vaccinologist (9, 10, 38,
39), does not seem to be totally applicable to OMV-based
vaccines, and we feel that this is the principal limitation in the
development of such a vaccine. The criteria are based on the necessity
of close contact between IgG antibodies (the main antibody class that
should be induced by an effective parenteral vaccine) in order to
activate complement; the relative dispersion of outer membrane proteins on the bacterial surface; and the relative inaccessibility of these
proteins, not only structural but also in the antigenic sense, created
by a nonxenogenic capsular B polysaccharide (8, 22, 38).
The IgG antibodies with bactericidal activity also have other important
biological functions (e.g., as opsonins), and the induction of
complement-fixing antibodies is more related to the Th1 pattern of
cytokine production (15). This implies that other
mechanisms could be present, such as IFN--mediated phagocyte
activation (28) in addition to bactericidal antibodies. That is why particular attention was given to the mechanism related to
the Th1 cellular response at the afferent and effector branches of the
immune response.
We have investigated antigen-specific immune responses after immunization with VA-MENGOC-BC. The cellular responses were measured by in vivo DTH and in vitro proliferation assays against OMVs, the main vaccine component. A strong DTH response was observed against the OMVs in all nursing babies after vaccination. All vaccinees, selected on the basis of low antibody levels against OMVs in order to obtain subjects as naive as possible (26), were positive in the LP assay after vaccination. Although the LP response observed was not very high, the presence of a strong DTH and the in vivo characteristic of this test mean that a functional cell-mediated immune response is induced. T-cell responses were also reported for humans immunized with the Norwegian (26) and Dutch (37) vaccines. The Norwegian vaccine is similar to VA-MENGOC-BC in its fundamental composition (both are OMV-based vaccines), but the Cuban vaccine has a twofold-higher protein content, N. meningitidis purified polysaccharide C is also present, it has a high concentration of A1(HO)3, it does not contain sucrose, and P4 and P5 are less represented (11, 42). The role of these differences and other components at the molecular level of immune induction has not been explored.
The influence of VA-MENGOC-BC immunization on the cytokine pattern of
PBMC from immunized subjects was evaluated after in vitro restimulation
with OMVs. The increase in IFN- and IL-2 mRNAs, but not in IL-4,
IL-5, or IL-10 mRNA, strongly suggests that a Th1 pattern of response
was stimulated at least in the six adult Cuban volunteers studied. The
first peak, observed after 14 h, might be related to the
complexity of the OMVs used as antigen for in vitro restimulation. The
characteristic wave of mRNA response could be related to the beginning
of protein synthesis and secretion or with transcriptional IFN- gene
regulation. IL-13 is a cytokine related to IL-4 and therefore
associated with Th2 responses, but this cytokine has no direct
influence on T cells (4, 6, 19, 32, 33).
At the effector level of the immune response, we evaluated the presence of antibodies with opsonic activity and the participation of other cells. An increase in opsonic activity was evident in immunized sera. In addition, the influence of complement on this activity is a well-known phenomenon confirmed in this study. Opsonins against N. meningitidis B have also been reported by others (15, 46). Opsonic activity was also detected in sera from subjects immunized with the Norwegian vaccine (1).
Neutrophils are important effector cells because they are the major
leukocytes present during the acute phase of inflammation, represent a
high percentage of human white blood cells, and have receptor for Fc
immunoglobulins, known to be effective at killing opsonized bacteria.
For that reason, the participation of PMN as effector cells was
evaluated. The in vitro experiment shows that nonactivated or activated
(LPS plus IFN-) cells were effective in killing N. meningitidis B, but more important, the elimination of PMN in
vivo by treatment with a specific MAb produced 100% mortality in
animals challenged with N. menigitidis B. This result suggests that PMN are essential in the defense against this infection, at least in rat models. It is important to note that peripheral blood
in the rat consists of only 25% PMN (15); thus, PMN may be even more influential in humans, where the percentage is higher (60 to 70%).
The importance of the Th1 pattern induced by VA-MENGOC-BC seems to
be relevant against N. meningitidis B infection, because high levels of IL-10 were associated with fatality in meningococcal disease (21) and the intrathecal production of IL-12 and
IFN- was observed in patients who had recovered from bacterial
meningitis (18).
The relevance of cell-mediated immunity in a Bordetella pertussis animal model has been demonstrated (23, 34). Recently, the importance of the Th1 response has also been reported for patients who have recovered from B. pertussis infection (40). In addition, the response induced by a protective vaccine in humans was also of Th1 pattern (41).
Even though the induction of a Th1-like pattern was demonstrated in this study, the majority of subjects were healthy Cuban adult volunteers; it would be appropriate to carry out a similar study of the primary response against VA-MENGOC-BC in a population of Cuban nursing babies, where the effects of environmental antigens can be decreased, or in other countries, where the circulation of Neisseria and other cross-reactive microorganisms is low, work that is in progress.
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ACKNOWLEDGMENTS |
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This work was supported by Finlay Institute.
We are indebted to E. LeRiverend for English corrections and to D. I. Stoot for criticism, suggestions, and English corrections.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Basic and Clinical Immunology, Finlay Institute, P.O. Box 16017, Havana City, Cuba. Phone: 53 (7) 217597 or 53 (7) 218321. Fax: 53 (7) 286075. E-mail: oliverp{at}finlay.edu.cu.
Editor: W. A. Petri Jr.
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REFERENCES |
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Abstract
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Materials and Methods
Results
Discussion
References
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Infection and Immunity, July 2001, p. 4502-4508, Vol. 69, No. 7
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.7.4502-4508.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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