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Infection and Immunity, September 1999, p. 4352-4359, Vol. 67, No. 9
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Host Responses to Recombinant Hemagglutinin B of
Porphyromonas gingivalis in an Experimental Rat
Model
Jannet
Katz,2,*
Kelley P.
Black,1 and
Suzanne M.
Michalek1,2
Departments of
Microbiology1 and Oral
Biology,2 School of Dentistry, The University
of Alabama at Birmingham, Birmingham, Alabama 35294
Received 22 February 1999/Returned for modification 26 April
1999/Accepted 5 June 1999
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ABSTRACT |
Porphyromonas gingivalis, a gram-negative,
black-pigmented anaerobe, is among the microorganisms implicated in
the etiology of adult periodontal disease. This bacterium possesses a
number of factors, including hemagglutinins, of potential
importance in virulence. Several hemagglutinin genes have been
identified, cloned, and expressed in Escherichia coli. The
purpose of this study was to characterize host responses to purified
recombinant hemagglutinin B (rHag B), using the conventional Fischer
rat as the experimental animal model. The effectiveness of immunization with rHag B on protection against experimental periodontal bone loss
following infection with P. gingivalis was also evaluated. Groups of rats were immunized by the subcutaneous route with rHag B in
complete Freund's adjuvant, immunized with rHag B and orally infected
with P. gingivalis, nonimmunized and noninfected, or orally
infected with P. gingivalis only. Serum and saliva samples were collected throughout the experiment and evaluated for serum immunoglobulin G (IgG) and IgM and salivary IgA antibody activity by
enzyme-linked immunosorbent assay. No salivary IgA anti-Hag B activity
was detected in the various groups of rats. A slight serum IgM response
similar to that seen in preimmune samples was observed. Serum IgG
antibody activity to Hag B was detected only in samples from rats
immunized with rHag B. This response was primarily of the IgG1 and
IgG2a subclasses, followed by IgG2b and low levels of IgG2c.
Supernatants from rHag B-stimulated splenic lymphoid cell cultures from
immunized rats contained high levels of gamma interferon, followed by
interleukin-2 (IL-2), IL-10, and then IL-4. These results are
consistent with the induction of T helper type 1 (Th1)- and Th2-like
responses. Western blot analysis of sera derived from rHag B-immunized
rats reacted with trichloroacetic acid (TCA) precipitates of P. gingivalis 33277, 381, A7A1-28, and W50, revealing a
50-kDa band reflective of Hag B. However, sera derived from rats
immunized with P. gingivalis whole cells or from rats
infected with P. gingivalis only did not react with rHag B
but did react with TCA precipitates of P. gingivalis
strains. Finally, radiographic measurements of periodontal bone loss
indicated that rats immunized with rHag B had less bone loss than
those infected with P. gingivalis only. These results demonstrate the effectiveness of purified rHag B in inducing a protective immune response and support the potential usefulness of
this component of P. gingivalis in the development of a
vaccine against adult periodontitis.
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INTRODUCTION |
Human adult periodontitis is an
infectious disease initiated and perpetuated by specific gram-negative
bacteria. Among these, the oral, black-pigmented anaerobe
Porphyromonas gingivalis has been accepted as an etiological
factor and thus implicated in the pathogenesis of the disease (10,
38, 39). This microbial pathogen has been commonly isolated from
periodontal diseased sites (26, 39, 40), and specific
antibodies to this bacterium have been found in patients with
periodontitis (29, 30, 45).
P. gingivalis possesses a number of potential virulence
factors thought to be important in the disease process (13, 28, 31, 33, 42). Among these are the hemagglutinins, nonfimbrial adhesins expressed on the surface of P. gingivalis.
Hemagglutinins have been implicated in virulence due to their ability
to agglutinate erythrocytes, which suggests that they may have a role
in adhesion to host tissues (12, 34). It is not yet known
how many different P. gingivalis hemagglutinins exist, and
there is no evidence as to their specific function. Early studies by
Inoshita et al. (14) reported the presence of three major
proteins in affinity-purified hemagglutinin preparations. Using
monospecific polyclonal and monoclonal antihemagglutinin antisera,
Mouton et al. (28) detected two major protein antigens in
immunoblots of cell surface extracts of P. gingivalis.
Extensive studies by Progulske-Fox et al. (34, 35) and
Lepine et al. (24, 25) described the cloning of four
P. gingivalis genes and their expression in
Escherichia coli. These genes encode for the proteins Hag A,
B, C, and D. Hag A and D have about 73.8% identity, whereas Hag B and
C are 98.6% homologous. However, neither shows significant homology to
Hag A. There are several genes encoding for hemagglutinin molecules, which may be an indication of their importance in virulence. Currently, Hag A and B have been more extensively characterized than Hag C or D. Furthermore, there has been a great deal of interest in the potential
utilization of Hag B in vaccine development. For instance, Dusek et al.
(6, 7) successfully expressed the hagB gene in an
avirulent strain of S. typhimurium. With the mouse as the
experimental animal model, humoral immune responses were evaluated
following the intragastric administration of the attenuated Salmonella strain. Both systemic and mucosal antibody
responses to Hag B were induced, thus demonstrating its immunogenicity. In a later study, it was shown that the subsequent administration of
the Salmonella strain to mice resulted in a recall response to Hag B in both serum and secretions (23). However, in
these studies, the involvement of the immune response in protection from periodontal disease was not determined. Thus, although the utilization of Hag B in vaccine development seems promising, an evaluation of its role in disease protection is essential.
Previous studies in our laboratory have shown that induction of
anti-P. gingivalis antibodies was associated with less bone loss in an experimental rat model, suggesting a role for specific antibodies in periodontal disease protection (18, 19).
However, the specificity of the protective antibody was not
established. The present investigation evaluated the humoral immune
response induced following subcutaneous (s.c.) immunization with
recombinant Hag B (rHag B) in an experimental rat model. Levels of
serum and salivary anti-Hag B antibodies were determined following
immunization and/or infection with P. gingivalis. We also
assessed the immunoglobulin G (IgG) subclass of the serum anti-Hag B
antibodies and the profile of T helper (Th) cytokines induced in rHag
B-stimulated splenic lymphoid cell cultures. Last, protection was
evaluated by radiographic assessment of periodontal bone loss.
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MATERIALS AND METHODS |
Animals.
Conventional Fischer CD F(344) rats used in this
study were bred and maintained in Trexler isolators and in horizontal
laminar flow units at the University of Alabama at Birmingham (UAB).
Animals were fed sterile diet L-485 (Harlan Teklad, Madison, Wis.) and were given water ad libitum throughout the experimental period. All
experiments were approved by the UAB Institutional Animal Care and Use Committee.
Bacteria.
P. gingivalis ATCC 33277, 381, A7A1-28
(ATCC 53977), and W50 were used in these studies. The bacteria were
cultured and maintained on enriched Trypticase soy plates consisting of
Trypticase soy agar supplemented with yeast extract (1%), 5%
defribinated sheep blood, hemin (5 mg/liter), and menadione (1 mg/liter) at 37°C in an anaerobic atmosphere of 10% H2,
5% CO2, and 85% N2 (43, 44). For
the preparation of P. gingivalis for various purposes including infection and for use as whole-cell (WC) coating antigen in
the enzyme-linked immunosorbent assay (ELISA), cultures were grown in
basal anaerobic broth (44) at 37°C under anaerobic conditions (17, 18). The bacteria were harvested, washed in sterile phosphate-buffered saline (PBS) (6,000 × g for
20 min), and resuspended in PBS. The estimated number of bacteria in
the suspension was determined by reading the optical density at 580 nm
and extrapolating from a standard curve. For oral challenge, the
bacteria was used immediately, whereas the bacteria to be used as
coating antigen in ELISA were suspended in sterile PBS containing
0.02% sodium azide (untreated) or 0.1% formalin (where stated) and
stored at 4°C until use.
TCA precipitation of bacterial proteins.
Freshly harvested
cultures of P. gingivalis 33277, 381, A7A1-28, and W50 were
washed twice with sterile PBS and resuspended in PBS to a final optical
density at 580 nm of 1.0. An aliquot of the suspensions (2 ml) was
centrifuged, and the pellet was resuspended in 0.5 ml 10%
trichloroacetic acid (TCA). Following overnight incubation at 4°C,
the precipitates were washed three times and then suspended in 0.05 ml
of distilled water. Phenylmethylsulfonyl fluoride (100 mM in
isopropanol) was added to 1 mM, and the TCA precipitates were stored at
4°C until use.
Hag B purification.
The hagB gene was cloned from
P. gingivalis 381 into a pET vector with a lac
promoter and histidine tag and expressed in Escherichia coli
JM109 (kindly provided by Ann Progulske-Fox and Thomas A. Brown,
University of Florida, Gainesville). A culture of E. coli was grown overnight at 30°C in Luria-Bertani (LB) broth containing ampicillin and kanamycin. An aliquot of the overnight culture was
transferred to LB broth with antibiotic supplements and incubated for 2 to 3 h at 30°C with vigorous shaking.
Isopropyl-
-D-thiogalactoside was added to a final
concentration of 1 mM, and the culture was incubated for an additional
3 h. The culture was centrifuged, and the pellet was resuspended
in binding buffer (5 mM imidazole, 0.5 M NaCl, 20 mM Tris-HCl [pH
7.9]) and stored at 
70°C. The cells were thawed, sonicated three
times, centrifuged, and passed through an 0.45-µm-pore-size filter.
Hag B was purified from the lysate by using a modified pET His · Bind system (Novagen, Madison, Wis.). The fraction containing rHag B
was dialyzed against PBS. The purity of rHag B was confirmed by Western
blot analysis using a rabbit anti-Hag B antibody (provided by Thomas A. Brown).
SDS-PAGE and Western blotting.
The reactivity of sera from
rats s.c.-immunized with rHag B or P. gingivalis 33277 WC or
of sera from rats infected with P. gingivalis 33277 against
rHag B or TCA precipitates of the various P. gingivalis
bacterial strains was assessed by sodium dodecyl sulfate-polyacrylamide
gel electrophoresis (SDS-PAGE) and Western blotting (19,
21). Briefly, samples were separated under dissociating conditions by SDS-PAGE (12.5% polyacrylamide), and the protein(s) was
transferred onto a nitrocellulose membrane by using the Mini Trans-Blot
electrophoresis system (Bio-Rad, Hercules, Calif.). The membrane was
blocked with 2% Tween 20 in wash buffer (50 mM Tris-HCl, 150 mM NaCl
[pH 10.2]) and washed three times with incubation buffer (wash buffer
containing 0.05% Tween 20). Following incubation for 2 h with rat
serum samples or with rabbit anti-Hag B antibody (provided by Thomas A. Brown), the membrane was washed three times and then incubated for 90 min with biotinylated goat anti-rat or anti-rabbit IgG followed by
streptavidin-alkaline phosphatase for the last 30 min. After washing,
the membrane was developed using
5-bromo-4-chloro-3-indolylphosphate-nitroblue tetrazolium tablets
dissolved in distilled water.
Experimental design.
Conventional Fischer rats (8 to 10 weeks old; six rats/group) were immunized s.c. once with rHag B (100 µg) in complete Freund's adjuvant (CFA) (group A), immunized s.c.
once with rHag B as described above and orally infected with P. gingivalis (group B), nonimmunized and noninfected (group C), or
orally infected with P. gingivalis only (group D). For oral
infection, freshly harvested P. gingivalis 33277 (approximately 1010 cells/ml) was mixed with 2%
carboxymethylcellulose, and individual rats were given 0.5 ml of the
suspension on day 13 following immunization by gastric intubation with
the aid of an intubation needle (2, 18, 19, 22). This
procedure was repeated twice at 24-h intervals. Sera and saliva samples
were collected from individual rats prior to the experimental period
and stored at 70°C until assayed by ELISA to determine baseline
antibody activity to rHag B and P. gingivalis WC antigens.
Starting on day 7 after immunization, sera and saliva were collected at
1- or 2-week intervals until the termination of the experiment (70 to
80 days after immunization). Samples were assessed for specific
antibody activity to rHag B and P. gingivalis WC by ELISA.
The levels of serum IgM, IgG, and IgG subclasses and of salivary IgA
antibody activity were determined. Selected serum samples were further
analyzed by Western blot for antibody activity to rHag B and to TCA
precipitates of the different P. gingivalis strains. At the
end of the experimental period, all rats were sacrificed, and their
spleens were removed, processed, and cultured to determine levels of
antigen-induced proliferative responses and cytokine production. The
mandibles from rats immunized and infected or infected only were then
removed for evaluation of periodontal disease by determining the amount
of bone loss by radiographic analysis. Control rat anti-P.
gingivalis WC serum samples were generated by s.c. immunization of
rats once with freshly harvested P. gingivalis 33277 (108) in CFA.
Sample collection.
Prior to the collection of serum and
saliva, rats were anesthetized by intramuscular injection (0.05 ml/100
g of body weight) of a solution of ketamine (100 mg/ml; Parke-Davis,
Morris Plains, N.J.) and xylazine (Tranquived; 1.5 mg/ml; VedCo, St.
Joseph, Mo.). Saliva (~1 ml) was collected over a 20-min interval
with a Pasteur pipette after intraperitoneal injection of carbachol (5 µg in 0.05 ml; Sigma Chemical Co., St. Louis, Mo.) and was clarified
by centrifugation (13,000 × g, 10 min, 4°C). Blood
was collected from the retro-orbital plexus throughout the experiment and by cardiac puncture at the termination of the experiment. The blood
was allowed to clot at 4°C, and the serum was collected after
centrifugation. All experimental samples were stored at 70°C until assayed.
Cytokines and proliferative responses.
The procedure used
for the preparation of splenic lymphoid cells was similar to that
previously described (8). Briefly, at the time of sacrifice,
spleens were aseptically removed, and single-cell suspensions were
prepared by mechanically dispersing the tissue through a sterile wire
mesh into RPMI 1640 (GIBCO Laboratories, Grand Island, N.Y.).
Erythrocytes were lysed with ammonium chloride buffer. The cells were
washed, suspended in warm (37°C) RPMI 1640 supplemented with 5%
fetal calf serum (FCS), and passed through a Sephadex G-10 (Pharmacia,
Piscataway, N.J.) column equilibrated with the same warm medium. The
eluted cell population was washed twice and suspended in RPMI 1640 supplemented with 2 mM L-glutamine, 100 U of penicillin per
ml, 10 µg of streptomycin per ml, and 10% FCS (complete medium) for
in vitro culture. Lymphoid cells were cultured in 96-well flat-bottom
plates (Falcon) in quadruplicate at 4 × 105 cells per
well. Cultures were incubated (37°C, 5% CO2) alone or
with various concentrations of concanavalin A (ConA; 5.0, 1.0, or 0.1 µg/ml), rHag B (10.0, 5.0, 1.0, or 0.1 µg/ml), or P. gingivalis 33277 WC (8 × 105, 4 × 105, or 2 × 105 WC/ml) for 48 h
(ConA) or 96 h (rHag B or WC). Cultures used to evaluate
proliferative responses were pulsed with [3H]thymidine
([3H]TdR; 0.5 µCi/well; Amersham Corp., Arlington
Heights, Ill.) during the last 18 h of incubation. Cells were
harvested onto glass fiber filters with a MASH II cell harvester
(Microbiological Associates, Walkersville, Md.), and the amount of
[3H]TdR incorporation was measured in a liquid
scintillation counter. The proliferative responses are expressed as a
stimulation index (SI) calculated as the mean level of
[3H]TdR uptake by cultures incubated with stimulant minus
the mean level of [3H]TdR uptake by the respective
control cultures which contain no stimulant, divided by the control
[3H]TdR uptake.
For cytokine analysis, cell cultures (2 × 105/well)
were prepared as described above, and the supernatants were harvested
at 72 h (ConA) or 96 h (rHag B). Immediately after
harvesting, the culture supernatants (CS) were stored at 70°C until
assayed. Cytoscreen immunoassay kits (BioSource International,
Camarillo, Calif.) were used to determine the concentration of gamma
interferon (IFN-
), interleukin-2 (IL-2), IL-4, and IL-10 in the CS.
Appropriate dilutions of CS were placed into 96-well microtiter plates,
previously coated with the appropriate anticytokine monoclonal antibody
(1 to 10 µg/ml). After incubation and washing, a biotinylated
antibody was added, following by streptavidin horseradish peroxidase
(HRP) and substrate, according to the manufacturer's directions. Color development was recorded at 450 nm, using a Vmax microplate
reader (Molecular Devices Corp., Menlo Park, Calif.) interfaced with a
Macintosh II computer (Apple Computer, Cupertino, Calif.). The final
concentrations of cytokines were calculated by interpolation of the
standard curves by using a four-parameter logistic algorithm. The lower
limits of sensitivity of the ELISAs used were 13 pg/ml for IFN-, 10 pg/ml for IL-2, 15 pg/ml for IL-4, and 20 pg/ml for IL-10.
Antibody responses.
Antibody activities to rHag B and
P. gingivalis WC were assessed by a previously described
ELISA (16, 18, 19, 37). Briefly, individual wells of
flat-bottom 96-well plates (Nalge Nunc International, Roshilde,
Denmark) were coated with rHag B or with P. gingivalis 33277 WC prepared in bicarbonate-carbonate buffer (pH 9.6; 100 µl; 1 µg
of rHag B per ml or 5 × 108 cells/ml) or with
anti-rat 
, µ, or heavy-chain antibody (UAB Immunochemical Core
Facility) or affinity purified anti-rat IgG1, IgG2a, IgG2b, or IgG2c
(The Binding Site Inc., San Diego, Calif.) in borate-buffered saline
(pH 8.2). Nonspecific binding sites were blocked with PBS containing
5% FCS (Gemini Bioproducts, Calabasas, Calif.) and 0.05% Tween 20 (pH
7.4) (Fisher Scientific, Fair Lawn, N.J.) for 2 h at room
temperature. From a starting dilution of serum (1:100 for IgM and IgG;
1:50 for IgG subclasses) or saliva (1:5 for IgA) prepared in PBS
containing 1% FCS and 0.1% Tween 20, five twofold dilutions were
added in duplicate to individual wells. Samples of serum and saliva
collected from individual rats throughout the experiment were assayed
for antibody activity, and all assays were repeated two or three times.
The levels of total salivary IgA and of salivary IgA and serum IgM and
IgG anti-Hag B or anti-P. gingivalis antibody activities
were determined by using standard curves generated with a calibrated
pool of Fischer rat serum with known amounts of the correspondent
immunoglobulins and wells coated with anti-rat , µ, or heavy-chain antibody (37) and are shown as geometric means
×/
standard deviation (SD). To quantitate IgG subclass antibody
activities in the experimental serum samples, a calibrated rat serum
(The Binding Site Inc.) with known amounts of the various IgG
subclasses was used to generate standard curves. After incubation (2 h
at 37°C) and washing of plates, biotin-conjugated anti-rat IgA, IgM,
or IgG (UAB Immunochemical Core Facility) or HRP-conjugated anti-rat
IgG subclass (The Binding Site Inc.) antibody was added to appropriate
wells. After overnight incubation (4°C), plates with biotinylated
anti-rat antibodies were washed and streptavidin-HRP (Southern
Biotechnology Associates, Inc., Birmingham, Ala.) was added for 30 min
at room temperature. All plates were washed, peroxidase substrate
[2,2'-azino-bis(3-ethyl-benzthiazoline-6-sulfonic acid)] in citrate
buffer (0.3 mg/ml, pH 4.0) containing 0.003% hydrogen peroxide was
added, and color development was recorded at 414 nm. The concentrations
(nanograms per milliliter) of specific anti-Hag B and anti-P.
gingivalis antibody activities were determined by assessing the
samples simultaneously with the calibrated pool of Fischer rat sera and
interpolating from a standard curve by using a four-parameter logistic algorithm.
Evaluation of periodontal bone destruction.
The amount of
periodontal bone loss was assessed by radiographic analysis as
previously described (18, 19). At the termination of the
experimental period, periodontal bone loss was assessed in rats
infected with P. gingivalis or in rats immunized s.c. (rHag
B) and infected in order to determine the effect of anti-Hag B
antibodies on protection against P. gingivalis infection.
The radiographic method assesses vertical bone loss, which is a linear measurement from the cementoenamel junction to the crest of the alveolar bone. Each mandible, with the lingual side down, was placed on
top of an intraoral film resting on a styrofoam platform. The radiation
source (Trophy model SU47 portable dental unit; Trophy Radiologie,
Vincennes, France) was positioned 25 cm from the film platform. A 10-mm
stainless steel dimensional reference was incorporated into each
radiographic image to ensure consistent magnification and to allow the
digital analysis to be expressed in millimeters of alveolar bone loss.
The radiographs were taken at 70 kV, 10 mA, and 0.10 s. The film was
developed through an automatic film processor. The radiographs were
analyzed by digital imaging methods (15). The radiographic
results are expressed as the amount of vertical bone loss in millimeters.
Statistics.
The significance of differences in antibody
activity, cytokine levels, and amount of bone loss between the
experimental and control groups was determined by analysis of variance
using StatView 4.0 software (Abacus Concepts, Berkeley, Calif.). A
P value of less than 0.05 was considered statistically significant.
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RESULTS |
Immune response to rHag B.
No salivary IgA antibody activity
to rHag B was detected in rats immunized by the s.c. route with rHag B
and/or infected with P. gingivalis. A slight serum IgM
response to rHag B was noted; however, the level of activity was
similar to that seen in preimmunization samples (data not shown). A
serum IgG anti-Hag B response was seen in the immunized (group A) and
the immunized and infected (group B) rats (Fig.
1). The kinetics of the responses were
similar in both groups of rats, although rats in group B had levels of antibody activity slightly lower than, but not statistically different from, levels in the group A rats. The responses peaked on day 40 and
persisted at a slightly lower magnitude until the termination of the
experiment. No serum IgG anti-Hag B antibody activity was detected in
the nonimmunized, noninfected (group C) or the nonimmunized, infected
(group D) rats. Further analysis of the IgG response to rHag B
indicated that the primary subclasses of antibodies induced were IgG1
and IgG2a (Fig. 2A) followed by IgG2b and
low levels of IgG2c (Fig. 2B). The IgG1, IgG2a, and IgG2b responses appeared to peak earlier in the group B rats than in the group A rats;
however, no significant difference in the IgG subclass responses
between the two groups of rats was seen.
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FIG. 1.
Serum IgG anti-Hag B activity in rats immunized s.c.
with rHag B (group A), in rats immunized s.c. with rHag B and orally
challenged with freshly harvested P. gingivalis 33277 (group
B), in nonimmunized, noninfected rats (group C), and in rats infected
only with P. gingivalis 33277 (group D). Values are the
geometric means ×/ SD of antibody activity in serum samples from six
rats/group. The results are from one experiment but representative of
two separate experiments.
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FIG. 2.
Serum IgG1 and IgG2a (A) and IgG2b and IgG2c (B)
responses to rHag B in rats immunized s.c. with rHag B (group A) and in
rats immunized s.c. with rHag B and orally challenged with freshly
harvested P. gingivalis 33277 (group B). Values are the
geometric means ×/ SD of antibody activity in serum samples from six
rats/group. The results are from one experiment but representative of
two separate experiments.
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Antigen-induced proliferative responses and cytokine
production.
Proliferative responses to rHag B were seen in splenic
lymphoid cell cultures from rats in groups A and B (Fig.
3A). Optimal stimulation to rHag B was
seen with a dose of 5 µg/ml in cultures from both groups of rats.
Cell cultures derived from rats immunized and infected showed a
slightly higher SI to all doses of rHag B tested than those derived
from immunized-only rats, although the difference was not significant.
Little or no proliferative response was seen when the cells from either
group of rats was stimulated with P. gingivalis WC (Fig.
3B). A slight stimulation was seen with 8 × 105
bacterial WC in cell cultures derived from immunized and infected rats.
Cell cultures from both groups of rats responded to ConA in a
dose-dependent manner (Fig. 3C). The response of cells from immunized
rats was higher than (but not significantly different from) that seen
with cells from immunized and infected animals.
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FIG. 3.
Proliferative responses to rHag B (A), P. gingivalis 33277 WC (B), or ConA (C) of splenic lymphoid cell
cultures derived from rats immunized s.c. with rHag B (group A; six
rats) or immunized with rHag B and infected with P. gingivalis 33277 (group B; six rats). Culture conditions were done
in quadruplicate, and the results are expressed as means of the SI,
determined as described in the text. The results are from one
experiment but representative of two separate experiments.
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Supernatants from lymphoid cells stimulated with rHag B and assayed for
the presence and level of cytokines revealed significantly
higher
(
P < 0.05) levels of IFN-
in the CS of cells
derived from
immunized and infected rats than in CS from cells derived
from
immunized-only animals (Fig.
4A).
The levels of IL-2 in the CS
from the immunized and infected group were
also significantly
higher (
P < 0.05) than those seen
in the CS from immunized-only
rats (Fig.
4B). IL-4 was detected in CS,
but in low amounts (Fig.
4C). The levels of IL-4 in supernatants of
rHag B-stimulated cell
cultures from immunized rats were slightly
higher than (but not
significantly different from) those seen in
cultures from immunized
and infected animals. Finally, the levels of
IL-10 detected in
the CS of rHag B-stimulated cells derived from
immunized and infected
rats were higher than but not significantly
different from those
seen in cultures from the immunized only group
(Fig.
4D).
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FIG. 4.
Quantitation of IFN- (A), IL-2 (B), IL-4 (C), and
IL-10 (D) in the supernatant of splenic lymphoid cultures derived from
rats immunized with rHag B or immunized with rHag B and orally
challenged with P. gingivalis 33277. Cultures were incubated
with rHag B (10 µg/ml). Values are the means ± standard errors
the means for cytokines in the supernatants of cultures derived from
six rats/group. The results are from one experiment but representative
of two separate experiments. *, Values are significantly different
(P < 0.05).
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Immune response to P. gingivalis WC.
To determine
if the anti-Hag B antibodies could react with P. gingivalis,
which could help determine the potential protective effect of these
antibodies against infection with this pathogen, serum samples from
rats immunized with rHag B were tested for reactivity against P. gingivalis WC by ELISA. The reactivity to WC of serum samples from
group A rats was 10- to 100-fold lower than that seen to rHag B (Fig.
5). Some antibody activity was seen in
serum samples when WC suspended in PBS were used as coating antigen,
whereas no increased in activity above baseline (day 0 sample) was seen
with WC treated with formalin. Serum samples from rats immunized by the
s.c. route with P. gingivalis WC had high levels of antibody
activity to formalin-treated P. gingivalis WC and
essentially no anti-Hag B antibody activity (Fig.
6). Similar results were obtained when
untreated P. gingivalis WC were used as coating antigen
(data not shown). Good serum IgG antibody responses to P. gingivalis WC were also seen in sera from rats in group D (data
not shown).
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FIG. 5.
Serum IgG responses to formalin or untreated P. gingivalis 33277 WC and to rHag B in rats immunized s.c. with rHag
B. Values are the geometric means ×/ SD of antibody activity in
serum samples from six rats/group. The results are from one experiment
but representative of two separate experiments.
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FIG. 6.
Serum IgG activity to formalin-treated P. gingivalis 33277 WC and to rHag B in rats immunized s.c. with
freshly harvested P. gingivalis 33277 in CFA. Values are the
geometric means ×/ SD of antibody activity in serum samples from six
rats/group. The results are from one experiment but representative of
two separate experiments.
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Western blot analysis of antibody responses.
Serum from rats
immunized with rHag B primarily reacted with a protein of the
approximate size of 50 kDa in the rHag B preparation and with the TCA
precipitates of P. gingivalis 33277, 381, A7A1-28, and W50
(Fig. 7A), indicating that Hag B is a
membrane component of these P. gingivalis strains. Sera from
rats immunized with P. gingivalis WC (Fig. 7B) or infected
with P. gingivalis only (data not shown) did not react with
rHag B but did react with TCA precipitates of P. gingivalis
33277, 381, A7A1-28, and W50.
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[in a new window]
|
FIG. 7.
(A) Immunoblot of serum samples from rats immunized by
the s.c. route with rHag B reacted with rHag B (lane 2) and TCA
precipitates of P. gingivalis 33277 (lane 3), 381 (lane 4),
W50 (lane 5), and A7A1-28 (lane 6). Lane 1, prestained
low-molecular-weight markers (in both panels, positions are indicated
in kilodaltons on the left). (B) Immunoblot of serum samples from rats
immunized by the s.c. route with P. gingivalis 33277 reacted
with rHag B (lane 2) and with TCA precipitates of P. gingivalis 33277 (lane 3), 381 (lane 4), W50 (lane 5) and A7A1-28
(lane 6). Lane 1, prestained low-molecular-weight markers.
|
|
Assessment of experimental periodontal bone loss.
At the end
of the experiment (days 70 to 80), the mandibles from individual rats
were removed and the amount of bone loss was quantified by the
radiographic technique (Fig. 8). Bone
loss in rats infected with P. gingivalis was significantly
greater (P < 0.05) than that in the animals which were
immunized with rHag B and then infected with P. gingivalis.
View larger version (29K):
[in this window]
[in a new window]
|
FIG. 8.
Periodontal bone loss on mandibular molars of rats
immunized with rHag B and infected with P. gingivalis 33277 and of rats infected with P. gingivalis 33277 only. Values
are the mean total amount of vertical bone loss ± SD as
determined by radiographic analyses. Data were collected from mandibles
removed from six rats/group between experimental days 70 and 80. The
results are from one experiment but representative of two separate
experiments. *, Values are significantly different (P < 0.05).
|
|
| |
DISCUSSION |
The purpose of this study was to characterize the immune response
induced following systemic immunization with purified rHag B and to
determine the effectiveness of the response in protection against
periodontal bone loss in an experimental rat model. When serum samples
from rats immunized by s.c. administration of rHag B in CFA were
assessed for antibody activity, a low level of IgM anti-Hag B activity
was detected. The level of activity was similar to that seen in
preimmune serum samples and in serum samples from nonimmunized,
noninfected animals, suggesting the presence of Hag B determinants
which have cross-reactivity with components of the indigenous
microorganisms in the rat. This finding was similar to our previous
observations on IgM anti-P. gingivalis activity in the rat
(19) and to what has been observed in periodontally involved
and control individuals (5). In contrast, a good serum IgG
anti-Hag B response was seen in rats immunized with the purified protein, demonstrating the immunogenicity of this molecule in the rat
model. These results extend the findings of Dusek et al. (6,
7) and Kohler et al. (23), who reported the induction of a systemic and mucosal response to this protein in mice following oral administration of a Salmonella typhimurium strain
expressing the cloned Hag B.
Analysis of the IgG subclass responses to rHag B in immunized or
immunized and infected rats indicated that IgG1 and IgG2a were the
primary IgG subclasses of antibodies induced, followed by IgG2b and a
very low level of IgG2c. In the murine system, Th2-like cells produce
IL-4, IL-5, and IL-10 and support an IgG1 subclass response, whereas
Th1-like cells produce IFN- and IL-2 and are involved in isotype
switching to IgG2a (9, 27, 41). The correlate of murine IgG1
in the rat is IgG1 and IgG2a, while murine IgG2a is homologous to rat
IgG2b (1). Therefore, the IgG subclass response pattern
observed in both groups of experimental animals would suggest a mixed
Th1 and Th2 response to systemically administered rHag B. The
production of IFN-, IL-2, IL-10, and some IL-4 by antigen-stimulated
splenic lymphoid cells from these rats supports the above observation.
At the time of cytokine assessment, cells from immunized and infected
rats produced significantly higher levels of IL-2 and IFN- than
cells from immunized-only rats. This finding suggests that infection
with P. gingivalis of immunized rats promoted the Th1-like
response pattern. The apparent earlier peak in the IgG2b response in
the immunized and infected rats compared to the immunized-only group
supports this possibility. Furthermore, previous studies in our
laboratory have shown that immunization with P. gingivalis
WC induced predominantly IgG2b antibodies, therefore indicating the
involvement of Th1-like cells (18). It is unclear why only
low levels of IL-4 were detected in the immunized animals since they
had high levels of IgG1 and IgG2a anti-Hag B antibodies reflective of a
Th2-like response pattern. Others have also reported the induction of a
dominant IgG1 antibody response in mice following immunization with an antigen and adjuvant, as well as high IFN- and low IL-4 production in vitro (46). It is possible that in our study the cytokine profile induced by rHag B in the splenic lymphoid cell cultures would
have revealed a higher level of IL-4 if cells were assessed shortly,
instead of 70 to 80 days, after immunization. It is also possible that
the amount of antigen induced IL-4 was sufficient to promote a Th2-like
response. Nevertheless, the finding of higher levels of IL-4 in the
immunized-only group than in the immunized and infected rats supports
the notion of a shift toward a Th1-like response upon P. gingivalis infection.
Kohler et al. (23), who analyzed the serum IgG subclass
distribution in mice following oral administration of a
Salmonella strain expressing the cloned Hag B, reported a
predominant systemic IgG2a anti-Hag B response. This predominant
Th1-like response pattern could have been influenced by the
Salmonella vector, as suggested by other investigators
(32, 47) who reported systemic Th1-like responses to cloned
antigens expressed by S. typhimurium. Conversely, our
laboratory reported a mixed Th1- and Th2-like response pattern to a
cloned antigen of Streptococcus mutans when expressed by
S. typhimurium (11). In this latter study,
responses to the purified S. mutans antigen were primarily
Th2-like. This finding suggests that the property of the cloned antigen
can influence the host immune response and that the nature of the
response is not entirely determined by the Salmonella
vector. This possibility gained support from our findings which
revealed a mixed Th1- and Th2-like response to purified rHag B even
when the antigen was administered in CFA, a condition which would favor
a Th1-like response. Further studies will be required to define
properties of cloned antigens and immunization regimens important in
influencing the nature of the specific host responses.
To determine the relevance of anti-Hag B antibodies in protection
against P. gingivalis pathogenesis, we next examined the ability of these antibodies to react with the bacteria. The amount of
reactivity to freshly harvested P. gingivalis was more than 10-fold lower than that seen to rHag B. This finding suggests that Hag
B antigenic epitopes are minimally expressed on the surface of P. gingivalis cells for induction of immune responses or that differences may exist in the antigenicity of native and rHag B. The
former possibility gains support from the finding that serum from rats
immunized s.c. with freshly harvested P. gingivalis contained a high level of antibodies reactive with WC but essentially no reactivity to Hag B. These serum samples, as well as those from rats
infected with P. gingivalis, also reacted with TCA
precipitates of the various P. gingivalis strains,
exhibiting a number of bands as has been previously shown (3,
20). Western blot analysis of serum samples from rats immunized
with rHag B revealed an antigen reactive band at ~50 kDa in TCA
precipitates of P. gingivalis 33277, 381, W50, and A7A1-28.
The band was similar to that seen with purified rHag B, as has been
previously reported by Progulske-Fox et al. (35) and Lepine
and Progulske-Fox (24), indicating that Hag B is a membrane
component of these P. gingivalis strains. Previous
studies have shown that purified Hag B inhibits hemagglutination of
sheep erythrocytes by WC of P. gingivalis 381 (7), implicating it as an adhesin. The results, taken
together, suggest that Hag B is not a dominant surface component
although it is sufficiently expressed to mediate hemagglutination and
therefore a relevant antigen for vaccine development.
It was of interest to see no increase above baseline in the level of
antibody activity to formalin-treated P. gingivalis WC in
serum samples from rats immunized with rHag B, suggesting that formalin
treatment altered surface components. Formalin treatment has been used
to inactivate bacterial toxins or to stabilize bacterial proteins for
vaccine preparations (4, 36). However, it has also been
suggested that formalin treatment can affect epitopes and influence the
nature of the immune response induced. In this regard, Di Tommaso et
al. (4) showed that some epitopes of formalin-treated
proteins of Bordetella pertussis were presented poorly or
not at all to T cells and ascribed this effect to a difference in the
ability of the formalin-treated compared to the native proteins to
undergo proteolytic processing.
Lastly, radiographic assessment of bone loss was done in rats infected
with P. gingivalis or immunized s.c. with rHag B and infected to determine the effect of anti-rHag B antibodies in protection against P. gingivalis infection. Animals orally
infected with P. gingivalis had significantly more bone loss
than rats that had been immunized with rHag B and then infected.
Therefore, these findings suggest that systemic antibodies to rHag B
were effective in protecting against the periodontal pathogen P. gingivalis. In a previous study (18), evidence was
provided suggesting a role for a systemic Th1-like response and for a
salivary IgA response to P. gingivalis WC in protection
against experimental periodontal bone loss. In the present study, a
salivary IgA anti-Hag B response was not detected, an expected finding
since the rats were immunized by a systemic and not a mucosal route.
Further studies will be required to establish the contribution of
salivary IgA anti-Hag B responses in protection against periodontal disease.
In summary, we have demonstrated that systemic immunization of rats
with purified rHag B in CFA results in the induction of a systemic but
not a mucosal salivary immune response. A mixed Th1- and Th2-like
systemic response was induced, as reflected by the serum IgG subclass
distribution of the anti-Hag B response and by antigen-specific
proliferative responses and antigen-induced cytokine production by
splenic lymphoid cell cultures from immunized animals. Finally, rats
immunized with rHag B were protected against experimental periodontal
bone loss following infection with P. gingivalis. These
results support the potential use of rHag B as a candidate antigen for
the development of a vaccine against periodontal disease.
| |
ACKNOWLEDGMENTS |
We thank Cecily Harmon for expertise in animal care and
radiographic measurements.
This study was supported by Public Health Service grants DE 10607, DE
08228, and DE 08182 from the National Institute of Dental and
Craniofacial Research.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Oral Biology, The University of Alabama at Birmingham, 845 South 19th St., BBRB 713/5, Birmingham, AL 35294-2170. Phone: (205) 934-2878. Fax:
(205) 934-1426. E-mail:
jenny_katz{at}micro.microbio.uab.edu.
Editor:
R. N. Moore
| |
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Abstract
Introduction
