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Infection and Immunity, September 1999, p. 4320-4325, Vol. 67, No. 9
Department of
Vaccinology1 and Department of
Environmental Medicine,2 National Institute
of Public Health, 0403 Oslo, Norway
Received 8 February 1999/Returned for modification 16 April
1999/Accepted 14 June 1999
In order to study the mucosal and serum antibody response to
polysaccharide-encapsulated bacteria in mice, a preparation of heat-inactivated Streptococcus pneumoniae type 4 was
administered, with and without cholera toxin, at various mucosal sites.
It appeared that intranasal immunization of nonanesthesized animals was
superior to either oral, gastric, or colonic-rectal antigen delivery
with regard to the induction of serum immunoglobulin G (IgG) and IgA, as well as saliva IgA antibodies specific for pneumococci. The marked
IgA antibody response in feces after intranasal, but not after oral or
gastric, immunization is suggestive of a cellular link between the
nasal induction site and the distant mucosal effector sites. Intranasal
immunization also induced antibodies in serum and in mucosal secretions
against type-specific capsular polysaccharide. IgA and IgG antibody
levels in pulmonary lavage fluids correlated well with saliva IgA and
serum IgG antibodies, respectively. Antibody determinations in
pulmonary secretions may therefore be redundant in some cases, and the
number of experimental animals may be reduced accordingly. After
intraperitoneal challenge with type 4 pneumococci, mice immunized
intranasally were protected against both systemic infection and death,
even without the use of cholera toxin as a mucosal adjuvant. Thus, an
efficient intranasal vaccine against invasive pneumococcal disease may
be based on a very simple formulation with whole killed pneumococci.
Streptococcus pneumoniae
is one of the major bacterial causes of respiratory tract infections
and a frequent cause of bacteremia (22, 25). With increasing
resistance of pneumococcal strains to antimicrobial agents
(7), there is a demand for preventive measures. The
presently available polyvalent polysaccharide vaccine offers protection
against a large number of pneumococcal strains, and it protects against
systemic pneumococcal infection (12, 24). However, the
protective efficacy against pneumonia is controversial (20,
28), and the polysaccharide vaccine is not considered to be
sufficiently immunogenic for use with infants and children under 2 years of age (21). There is thus a need for alternative vaccination strategies, e.g., development of polysaccharide-protein conjugate vaccines, pneumococcal protein vaccines, or mucosal vaccines.
Most pathogens enter the host through the mucosal membranes and seem to
induce a local mucosal immune response, mainly represented by secretory
IgA (10). Studies of carriage of pneumococci in the upper
respiratory tract have shown that such carriage may induce
anti-pneumococcal antibodies (15). In preliminary studies with mice, we have been able to show that a preparation of whole heat-inactivated pneumococci was immunogenic when applied to mucosal surfaces and that the nasal mucosa may be the preferred site for antigen delivery (2). It has also been shown recently that nasal immunizations with pneumococcal surface protein A could induce
immunity with the power to protect against challenge with pathogenic
organisms (27).
Most previous studies were done with cholera toxin (CT) or its nontoxic
subunit B as a mucosal adjuvant (8, 23, 26, 27). However, it
became clear from other experiments that several killed airway
pathogens, i.e., Bordetella pertussis, group B streptococci, and outer membrane vesicles from group B meningococci, were strongly immunogenic when given as a nasal vaccine, even without the use of CT
(9, 14, 16, 18). If this is also valid for whole inactivated
pneumococci, it may be possible to create nonproliferating mucosal
vaccines without additional mucosal adjuvants, which might themselves
be immunogenic or tolerogenic (13).
The aim of this study was to determine in more detail the mucosal site
that would be the most efficient for induction of systemic and mucosal
antibody responses after application of heat-inactivated whole
pneumococci. We also attempted to find out whether cholera toxin would
be necessary as a mucosal adjuvant for the whole pneumococcal vaccine.
Finally, we used a systemic-infection model to test the protective
effect of this vaccine when administered on the appropriate mucosal site.
Bacteria.
A human isolate of S. pneumoniae
serotype 4 was used for immunization and challenge. Heat-killed
bacteria for immunization were prepared by culturing pneumococci in
Todd-Hewitt broth (Difco Laboratories, Detroit, Mich.) with 17% fetal
calf serum (Gibco Laboratories, Life Technologies Ltd., Paisley,
Scotland) for 18 h at 36°C in 5% CO2, after which
they were centrifuged and washed three times in sterile pyrogen-free
saline (3). The number of bacteria in the final suspension
was determined by plating 10-fold serial dilutions onto horse blood
agar plates. Heat inactivation was accomplished in a water bath at
56°C for 30 min. No live bacteria were detected after this suspension
was plated onto agar plates.
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Copyright © 1999, American Society for Microbiology. All rights reserved.
Intranasal Immunization with Heat-Inactivated
Streptococcus pneumoniae Protects Mice against Systemic
Pneumococcal Infection
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
70°C, ready for challenge experiments
after thawing and appropriate dilution.
Animals. Inbred female BALB/cABom mice, 7 to 9 weeks old, were obtained from Gl. Bomholtgård Ltd. Ry, Denmark. Outbred female HsdOla:NIHS mice, 6 to 8 weeks old, were obtained from Harlan Olac Ltd., Oxon, United Kingdom. They were all specific-pathogen-free mice and were housed in cages with six to eight mice each with Beekay GLP bedding (B & K Universal AS, Nittedal, Norway) under standard conditions with regulated day length, temperature, and humidity. Tap water and pelleted food (Ewos-Alab R3, rats and mice; Ewos AB, Södertälje, Sweden) were offered ad libitum. The experiments were performed in conformity with the laws and regulations controlling experiments with live animals in Norway and were approved by the local officer of the Experimental Animal Board under the Ministry of Agriculture of Norway.
Immunizations. In the first experiment, groups of six BALB/c mice were immunized four times at weekly intervals, each group at a different mucosal site (intranasal, oral, intragastric, and colonic-rectal). No anesthetics were given in this first experiment. Each dose of antigen solution corresponded to a mixture of 25 µl of the heat-inactivated pneumococci (1010 CFU/ml before heat inactivation) and 5 µl (1 mg/ml) of CT (Calbiochem Corp., La Jolla, Calif.). The intranasal immunization was carried out with the mouse held in a supine position with the head down while 30 µl of the antigen solution was delivered slowly with a micropipette onto the nares so that the mouse could sniff it in. For oral immunizations, the antigen solution was given slowly with a micropipette so that the mouse could suck the fluid from the tip. The antigen solution to be given intragastrically was mixed with 150 µl of 0.1 M NaHCO3 (pH 8.1), making up 180 µl per dose, which was given intragastrically with a blunt steel feeding tube. For colonic-rectal immunization, 30 µl of the antigen solution was delivered by a feeding tube inserted via the anus with the tip approximately 3 cm from the anal opening.
In the second experiment, groups of NIHS mice were immunized intranasally four times at weekly intervals with 25 µl of heat-inactivated pneumococci, either mixed with or without added CT. These mice were briefly anesthetized intravenously with 0.01 ml (10 mg/ml) of propofol (Diprivan; Zeneca Ltd., Macclesfield Cheshire, United Kingdom) before intranasal immunization, which was performed as described for the first experiment. The mice recovered completely 1 to 2 min after anesthesia. Groups of mice given anesthesia and 25 µl of pyrogen-free saline intranasally served as controls.Collection of samples for antibody determinations.
Blood was
obtained from the lateral femoral vein in heparinized capillary tubes
(Vitrex, Herlev, Denmark) and was separated and stored at 20°C
until it was analyzed (4). Saliva and feces were collected,
and extracts were made as described previously (17).
Briefly, saliva was collected by inserting the tips of absorbent
cylindrical wicks (2 by 25 mm) (Polyfiltronics Group Inc., Rockland,
Mass.) into the mouths of mice immediately after salivation was induced
by a single intraperitoneal injection of 0.1 mg of pilocarpin-HCl
(Sigma Chemical Co., St. Louis, Mo.) in 100 µl of phosphate-buffered
saline (PBS). The weight of the collected secretions was calculated as
the difference between the weights of the wicks before and after
collection. Two wicks saturated with saliva were obtained from each
mouse, frozen at 20°C in 1.5-ml microcentrifuge tubes, and
subsequently extracted with 500 µl of PBS containing 5% nonfat dry
milk (Oxoid skim milk powder; Unipath Ltd., Basingstoke, Hampshire,
England) and the following protease inhibitors: 0.2 mM
4-(2-aminoethyl)-benzenesulfonylfluoride (AEBSF) (Calbiochem), 1 µg
of aprotinin/ml, 10 µM leupeptin (both from Sigma), and 3.25 µM
bestatin (Boehringer Mannheim, Indianapolis, Ind.). After being
vortexed twice for 15 s, the tubes were centrifuged at
16,000 × g for 2 min at 4°C to drive fluid out of
the wicks.
20°C, and subsequently vacuum
dried in a Speed Vac concentrator (Savant Instruments, Inc.,
Farmingdale, N.Y.). After the net dry weights were recorded, extracts
were made by adding 20 µl of PBS, with dry milk and protease inhibitors, per mg of dry feces, followed by extensive vortexing and
centrifugation at 16,000 × g for 2 min at 4°C
(17). The clear supernatants were used for further analyses.
Immediately after the animals were killed, lung lavage fluid was
obtained by a single injection into the trachea of 1.5 ml of PBS,
followed by aspiration through a 25-G needle. Possible backflow of
saline during this procedure was prevented by tying off the proximal
part of the trachea.
In the first experiment, all samples except lung lavage fluids were
collected before and 1 week after the fourth immunization. In the
second experiment, samples were also collected just before the third
immunization and on the day before bacterial challenge. Blood for
bacterial counts was obtained 3, 12, 24, 48, and 72 h after
challenge. Unless otherwise specified, all samples and extracts
intended for antibody analyses were stored at 20°C until they were analyzed.
Quantitation of anti-pneumococcal antibodies.
Immunoglobulin
M (IgM), IgG, and IgA antibodies to pneumococcal polysaccharide
(anti-PPS) serotype 4 were determined by enzyme-linked immunosorbent
assay (ELISA) with Nunc (Roskilde, Denmark) Immuno plates (no. 269787)
as previously described (5). Briefly, the plates were coated
by incubation with PPS serotype 4 (American Type Culture Collection,
Rockville, Md.). Plasma samples were neutralized with pneumococcal C
polysaccharide to remove activity against this pneumococcal antigen and
tested at a dilution of 1:100 (5). Secretions were tested at
a dilution of 1:50. A pool of sera from immunized mice was included on
each plate as a positive control. Alkaline phosphatase (ALP)-conjugated
goat anti-mouse IgM, IgG, or IgA (µ, 
, and 
chain specific,
respectively) (Sigma Chemical Company) was used as a conjugate.
Experimental infections. In the second experiment, the mice were challenged by intraperitoneal injection of live pneumococci according to a previously described infection model (1). The mice were challenged 1 week after the last immunization, and a challenge dose 10 times the 50% lethal dose (LD50) for this serotype, i.e., approximately 20 to 30 CFU per mouse, was given. The number of bacteria in the inoculum was confirmed by plating 100 µl from serial 10-fold dilutions onto blood agar plates. The number of bacteria in the blood of infected animals was determined by applying 25-µl volumes of similar 10-fold dilutions of blood to the plates. Colonies of bacteria were counted after incubation at 36°C in a 5% CO2 atmosphere for 18 h. The challenged mice were observed twice daily by an experienced person, and signs of sickness and dead mice were recorded. Moribund animals, which it was assumed were going to die within a few hours, were sacrificed by cervical dislocation for humane reasons. Mice still alive after 14 days were considered to have survived the infection.
Statistical analysis. Statistical analysis was performed with SigmaStat statistical software (version 3.01; Jandel Scientific, Erkrath, Germany). The nonparametric Mann-Whitney U test, the chi square test, and the Fischer exact test were used. The limit of statistical significance used was a P value of 0.05.
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RESULTS |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Nasal immunizations are most efficient for induction of systemic
and mucosal antibodies.
To find the most efficient means of
applying mucosal vaccines consisting of whole killed pneumococci,
groups of mice were immunized via the nasal, oral, gastric, or rectal
route. It was evident from the results of this experiment that the
nasal route, with CT as a mucosal adjuvant, was by far superior to any
other route for induction of serum IgG antibodies to whole pneumococci (Table 1). No such antibody response was
elicited when the pneumococcal antigen was given via other routes, even
when antigen was given directly into the stomach with bicarbonate to
neutralize the gastric acid. However, all immunized mice belonging to
any group developed strong serum IgG antibodies to CT (results not
shown). In the second experiment, in which whole killed pneumococci
were given intranasally with or without CT, levels of serum IgG and IgM
antibodies to whole pneumococci were markedly higher in mice which were
given pneumococci with CT than in those given pneumococci without CT (data not shown).
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IgA antibodies in saliva and IgG antibodies in serum correlate with the corresponding antibodies in pulmonary lavage fluid. Only low concentrations of IgA antibodies to pneumococci were found in lung lavage fluid. Still, a significant increase in IgA antibodies was observed in the lung lavage fluid in the groups of mice which had been immunized via the nasal or oral route (Table 2). Moreover, the concentration of IgA antibodies in lung lavage fluid correlated well with the concentration of IgA antibodies in saliva (Fig. 1, upper panel) (r = 0.89; P < 0.0001) but with concentrations roughly 10 times less than those in saliva. On the other hand, IgA antibody concentrations in lung lavage fluid did not correlate significantly with serum IgA concentrations.
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Nasal immunization with whole killed pneumococci can induce
antibodies to PPSs.
In the first immunization experiment, with the
use of CT as a mucosal adjuvant with BALB/c mice, IgG antibodies to PPS
could not be detected in serum or secretions. However, significant
increases in serum IgA antibodies to PPS could be demonstrated after
nasal, oral, gastric, and rectal immunization (Table
3). On the other hand, extracts of feces
were the only kind of sample representing secretions in which such IgA
antibody responses could be demonstrated, and then only after nasal and
rectal antigen deliveries (Table 3). Significant increases in serum IgM
antibodies to PPS were detected after intranasal oral, gastric, and
rectal immunization, but no IgM antibodies to PPS could be demonstrated
in any secretion (results not given).
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0.01 and P < 0.001, respectively) (Fig. 2). Some
mice showed an increase in IgA antibody levels, but the increase was
not statistically significant. When pneumococci alone were used for
nasal immunizations, however, only IgM antibodies to PPS were increased
(P < 0.001). Moreover, there was no significant
difference in the IgM antibody levels whether or not CT was added to
the antigen solution (Fig. 2).
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Nasal immunizations with whole killed pneumococci can protect against systemic pneumococcal infection. The groups of mice which had been immunized intranasally as part of the second experiment, and which were given lethal doses of viable pneumococci intraperitoneally, were examined for viable bacteria in the blood. As early as 3 h after the bacterial challenge, the animals which had been immunized with the pneumococcal preparation had significantly (P = 0.01) fewer bacteria than those which had been given only saline as a nasal placebo vaccine (Fig. 3). It made no difference whether CT had been given together with the killed pneumococci. This difference in bacterial counts between control animals and animals which had been given pneumococci with or without CT was even more pronounced at 12 h after the bacterial challenge (P = 0.001).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this study, we have shown that whole heat-inactivated pneumococci can induce both systemic and mucosal antibodies when applied on various mucosal surfaces. Results of our first experiment indicate that intranasal application of this antigen, plus CT as a mucosal adjuvant, was superior to the oral, gastric, and rectal routes of antigen delivery (2). It was also evident that immunization via these alternative routes was not able to induce anti-pneumococcal IgG antibodies, which might be crucial for protection against systemic disease. However, IgG antibodies against CT were induced after immunization at all mucosal sites. The induction of systemic immunity to pneumococci via the nasal route suggests that the nasopharyngeal mucosa possesses the necessary structures to make mucosal immunizations a realistic alternative to the use of parenteral vaccines (11).
The superiority of nasal versus oral, gastric, and rectal routes of antigen presentation was confirmed by the demonstration of specific IgA antibodies in serum and samples representing secretions. The demonstration of IgA antibodies in secretions after the antigen was given orally, and not gastrically, might thus be explained by the antigen in the first case having reached the nasopharyngeal induction sites. Furthermore, only intranasal immunizations, in addition to rectal antigen delivery, induced significant increases in intestinal IgA antibodies, as reflected in extracts of feces. This was surprising, considering the fact that neither oral nor gastric immunizations with the same antigen were able to induce significant increases in such intestinal antibodies. The lack of intestinal antibodies after oral and gastric immunizations indicates that induction of intestinal antibodies after intranasal immunization was not due to swallowing or leakage of antigen from the nose into the intestines. The stimulus for antibodies to be produced locally in the gut is therefore suggestive of a cellular link between the nasal induction site and the intestinal effector site.
Our finding of IgG as well as IgA antibodies to pneumococci in lung lavage fluid, especially after nasal immunization, might indicate that both these antibodies have a barrier function against invasive pneumococci. The IgG antibodies in the pulmonary lavage fluids also seemed to mirror antibodies in serum, from which they are probably derived. Similarly, we have recently showed that IgG antibodies to B. pertussis in pulmonary secretions reflected the corresponding serum antibodies, which were initiated by nasal immunization (9). A protective effect of systemic antibodies against pulmonary infections might thus be conferred all the way from the tissue fluid to the mucosal surfaces.
The present finding that pulmonary IgA antibodies to pneumococci correlated with such antibodies in saliva indicates that at least some of the IgA is produced locally in the lungs to contribute to this presumed surface protection. It seems, therefore, that the IgA antibodies in saliva reflect the IgA antibodies in the lung secretions and that analyses of salivary IgA would be sufficient for evaluation of mucosal airway antibodies. Since saliva samples can be collected several times from the same animal, there is less need for collection of pulmonary secretions, and the number of mice used for experimental purposes can be reduced.
In the second experiment, significant increases of serum anti-polysaccharide IgG and IgM were induced in NIHS mice, whereas only serum IgM antibodies were induced in the first experiment with BALB/c mice. Parenteral immunization of BALB/c mice with PPS, conjugate vaccine, or heat-inactivated pneumococci also seems to induce serum IgM and no IgG antibodies (3, 5, 19). In other strains of mice, however, IgG antibodies can be induced after parenteral immunization with a pneumococcal conjugate vaccine (19), and low levels of IgG antibodies may even be induced in NIHS mice after immunization with polysaccharides alone (unpublished observations). The discrepancy in antibody responses in the first versus the second experiment may therefore be due to the use of different strains of mice.
Intranasal immunization with PPS type 3 containing liposomes has also been shown by others to induce IgA antibodies specific for type 3 polysaccharide in lung lavage fluid (6). In addition, we have now shown that both nasal and rectal immunizations induced intestinal IgA antibodies directed against the homologous type of polysaccharide. To some extent, however, these intestinal antibody responses to the polysaccharide antigens after mucosal immunization seemed to depend on the use of strong mucosal adjuvants, such as CT, and it remains to be shown whether polysaccharides as part of a mucosal vaccine induce protective immunity.
The intranasally immunized mice in the present study were well protected against lethal intraperitoneal challenge with live pneumococci. This was evident also with a vaccine consisting of only killed whole pneumococci, i.e., without additional mucosal adjuvants, despite the fact that some mice developed only low levels of antibody to polysaccharides in the serum. A similar discrepancy between low levels of ELISA antibodies specific for serotype 4 polysaccharide and protection against pneumococci of the same serotype has also been observed in other studies (4, 19). As opposed to antibodies against polysaccharides, in the present study, intranasal immunization induced strong antibody responses to whole pneumococci in all mice, even without CT. Antibodies to pneumococcal antigens other than polysaccharide antigens may therefore have contributed to protection. Since such antigens may be common to many pneumococcal serotypes, one could speculate whether a pneumococcal whole-cell vaccine given intranasally would protect against infections caused by several other serotypes.
The present finding that CT was not necessary for a nasal whole-cell vaccine to induce effective antibodies is in accordance with results of studies with outer membrane vesicles from meningococci (14). Recently, it has been found that CT actually inhibited the antibody responses to whole group B streptococci (18) and to B. pertussis (9) that had been given intranasally. It may thus be possible to create effective nonproliferating mucosal vaccines based on very simple formulations.
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ACKNOWLEDGMENTS |
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We thank Else-Carin Groeng, Inger Lise Haugen, Rita Bente Leikvold, Gro Lermark, and Trude Olsen for invaluable help and excellent technical assistance and Morten Harboe for inspiring discussions.
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FOOTNOTES |
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* Corresponding author. Mailing address: National Institute of Public Health, Department of Vaccinology, P.O. Box 4404 Torshov, N-0403 Oslo, Norway. Phone: 47 22 04 23 56. Fax: 47 22 04 23 01. E-mail: ingeborg.aaberge{at}folkehelsa.no.
Editor: J. R. McGhee
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REFERENCES |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Infection and Immunity, September 1999, p. 4320-4325, Vol. 67, No. 9
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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