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Infect Immun, June 1998, p. 2587-2594, Vol. 66, No. 6
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Volatile Fatty Acid, Metabolic By-Product of
Periodontopathic Bacteria, Induces Apoptosis in WEHI 231 and RAJI B
Lymphoma Cells and Splenic B Cells
Tomoko
Kurita-Ochiai,*
Kuniyasu
Ochiai, and
Kazuo
Fukushima
Department of Microbiology, Nihon University
School of Dentistry at Matsudo, Matsudo, Chiba 271, Japan
Received 18 November 1997/Returned for modification 5 February
1998/Accepted 16 March 1998
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ABSTRACT |
The ability of butyric acid, an extracellular metabolite from
periodontopathic bacteria, to induce apoptosis in murine WEHI 231 cells, splenic B cells, and human RAJI cells was examined. The culture
filtrate of Porphyromonas gingivalis,
Prevotella loescheii, and Fusobacterium
nucleatum, which contains high a percentage of butyric
acid, induced DNA fragmentation in WEHI 231 cells. Volatile fatty acid,
especially butyric acid, significantly suppressed B-cell viability in a
concentration-dependent fashion. The DNA fragmentation assay indicated
that butyric acid rapidly induced apoptosis in WEHI 231 cells (with
1.25 mM butyric acid and 6 h after treatment), splenic B cells
(with 1.25 mM butyric acid), and RAJI cells (with 2.5 mM butyric acid).
Incubation of WEHI 231 cells with butyric acid for 16 h resulted
in the typical ladder pattern of DNA fragmentation and the
apoptoic change such as chromatin condensation and hypodiploid
nuclei. Cell cycle analysis implied that butyric acid arrested the
cells at the G1 phase. The inhibitory assay suggested that
butyric acid-induced apoptosis of WEHI 231 and splenic B cells
was inhibited by W-7, a calmodulin inhibitor. These results suggest
that calmodulin-dependent regulation is involved in the signal
transduction pathway of butyric acid.
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INTRODUCTION |
It is recognized that periodontal
diseases are infectious and that periodontal tissue breakdown results
from the interaction of specific anaerobic bacteria and host immune
mechanisms. A recent study indicates that severe destructive adult
periodontitis is a multibacterial infection and that certain
combinations of periodontopathogens, namely, Porphyromonas,
Prevotella, and Fusobacterium spp., seem to be
important in the pathogenesis of the disease (43). These bacteria produce an elaborate variety of virulence factors such as
proteases, lipopolysaccharides, and fimbriae (42).
The metabolism of each of these bacteria is also characterized by the
production of an identifiable pattern of short-chain fatty acids, which
are major by-products of anaerobic metabolism that are released into
the microenvironment at the infection site (18) and can
diffuse across biological membranes (40). Previous studies
have demonstrated that these fatty acids exert inhibitory effects on
gingival fibroblast proliferation (41), colon cancer cell
growth (15), and phagocytosis (12, 37). Our
previous study (23) demonstrated that short-chain fatty
acids, especially volatile fatty acids present in the culture filtrates
of Porphyromonas gingivalis, Prevotella
loescheii, and Fusobacterium nucleatum, greatly
inhibited murine T- and B-cell proliferation and cytokine production by
concanavalin A-stimulated splenic T cells. Furthermore, we found that a
representative volatile fatty acid, butyric acid, induced cytotoxicity
and apoptosis in murine thymocytes, splenic T cells, and human
Jurkat T cells (24).
Apoptosis is an active process controlled by intracellular regulatory
systems. For example, it is suggested that in several apoptotic
systems, intracellular signal-transducing systems, e.g., protein
phosphorylation and Ca2+ signaling, are involved in the
control of the induction of DNA fragmentation (16, 39). In
this study, we report that culture filtrates of periodontopathic
bacteria and butyric acid present in the filtrate induce
apoptosis in murine WEHI 231 cells, splenic B cells, and human
RAJI cells. To understand better the intracellular mechanism of the DNA
fragmentation in this system, we examined the effects of several kinds
of specific modulators of cell functions on DNA fragmentation.
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MATERIALS AND METHODS |
Bacterial strains and culture conditions.
P.
gingivalis W83 and ATCC 33277, P. loescheii ATCC
15930, Prevotella intermedia ATCC 25261 and 25611, F. nucleatum JMC 8532 and ATCC 23726, Actinobacillus
actinomycetemcomitans Y4, and Capnocytophaga ochracea
ATCC 33596 were used in this study. P. gingivalis W83 was kindly provided by K. Okuda, Tokyo Dental College, Tokyo, Japan.
P. gingivalis, P. loescheii, and
P. intermedia were separately grown in brain heart
infusion (BHI) broth (Difco Laboratories, Detroit, Mich.) supplemented
with 5% bovine serum, 5 µg of hemin per ml, and 0.4 µg of menadion
per ml in a model 1024 anaerobic system (Forma Scientific, Marietta,
Ohio) for 2 days. A. actinomycetemcomitans, C. ochracea, and F. nucleatum were grown in BHI broth
supplemented with 5% bovine serum, at 37°C for 2 days in a 5%
CO2 atmosphere.
Preparation of bacterial culture filtrates.
The cultures
were incubated for 2 days and centrifuged at 10,000 × g for 20 min at 4°C. The pH of the 48-h P. gingivalis, P. loescheii, P. intermedia, and F. nucleatum spent media ranged from 6.5 to 6.8, while the pH of A. actinomycetemcomitans and C. ochracea spent media
ranged from 6.0 to 6.3. The supernatant fluid was removed, adjusted to
pH 7.0, and sterilized by filtration through a 0.22-µm-pore-size
membrane filter (Millipore Corp., Bedford, Mass.). A pH-adjusted
sterile BHI medium was used as control.
Short-chain fatty acid.
Highly purified butyric, propionic,
and isovaleric acids were purchased from Sigma Chemical Co. (St. Louis,
Mo.). Solutions of fatty acid ranging in concentration from 0.15 to 5 mM were diluted in RPMI 1640 (Gibco Laboratories, Grand Island, N.Y.) medium and adjusted to pH 7.2 with sodium hydroxide.
Mice.
C3H/HeN mice were obtained from Charles River Breeding
Laboratories (Kanagawa, Japan). The mice were maintained in the Animal Facility of Nihon University School of Dentistry at Matsudo under standard care and given food and water ad libitum. Female and male mice
were used at 9 to 10 weeks of age.
B-cell preparation.
Spleens were aseptically removed, and
single-cell suspensions were prepared by gently teasing the cells
through sterile stainless steel screens. Preparations of B cells from
mouse spleens were obtained as described previously (23).
Briefly, splenic cell suspensions were treated with a cocktail of
monoclonal antibodies (rat anti-mouse Thy 1.2, anti-Lyt2, and anti-L3T4
antibodies) for 30 min at 4°C, followed by incubation with rabbit
anti-rat immunoglobulin G and complement (Low Tox rabbit complement;
Cedarlane Laboratories Ltd., Ontario, Canada) for 30 min at 37°C.
This purified B-cell preparation contained less than 2%
Thy-1+ cells, as determined by immunofluorescence with a
FACScan fluorescence-activated cell sorter (Becton Dickinson and Co.,
Sunnyvale, Calif.). The B lymphoma cell lines WEHI 231 (mouse) and RAJI
(human) were obtained from Japan Cancer Research Resources Bank. These
cells were cultured at 37°C in a moist atmosphere of 5%
CO2 in complete medium consisting of RPMI 1640 supplemented
with 10% heat-inactivated fetal calf serum, 2 mM
L-glutamine, 100 U of penicillin per ml, 100 µl of streptomycin per ml, and 0.05 mM 2-mercaptoethanol.
Cell proliferation assay.
As a method of assessing cellular
proliferation following the addition of fatty acid, the colorimetric
MTT [3-(4,5-dimethyl-2-thiazoyl)-2,5-diphenyl tetrazolium bromide;
Sigma) assay was performed (21). In viable cells, the
mitochondrial enzyme succinate dehydrogenase can metabolize MTT into a
formazan dye that absorbs light at 550 nm. WEHI 231 and RAJI cells were
seeded at a density of 2.0 × 105 cells per well in
0.1 ml of complete medium in flat-bottom 96-well plates. Butyric,
propionic, and isovaleric acids in RPMI 1640 were added to a final
concentration of 0.15 to 5 mM, and each concentration of fatty acid was
tested in quadruplicate. After incubation for 42 h, 20 µl of MTT
(5 mg/ml in phosphate-buffered saline [pH 7.2]) was added to each
well. Following 6 h of incubation, the supernatants were decanted,
and the formazan precipitates were solubilized by the addition of 150 µl of 100% dimethyl sulfoxide (Sigma) and placed on a plate shaker
for 10 min. Absorbance at 550 nm was determined on a Corona MT32
spectrophotomeric microplate reader (Corona Electric Co., Ibaraki,
Japan). The absorbance of the untreated cultures was set at 100%. The
mean relative absorbance and the standard error of the mean (SE) were
calculated for every concentration of fatty acid tested.
B-cell culture for apoptosis.
B cells were suspended
in complete medium. Cells (4.0 × 106 per well for
splenic B cells and 106 per well for WEHI 231 cells and
RAJI cells) were cultured in 1 ml of medium in 24-well tissue culture
plates (Falcon; Becton Dickinson Labware, Lincoln Park, N.J.) in the
presence or absence of various concentrations of butyric acid or 100 µl of culture filtrates. At the times indicated in the figures, cells
were harvested and centrifuged at 400 × g for 5 min
and washed twice with ice-cold phosphate-buffered saline. Cells were
resuspended in 400 µl of hypotonic lysis buffer (0.2% Triton X-100,
10 mM Tris, 1 mM EDTA [pH 8.0]) and centrifuged for 15 min at
13,800 × g (31). Half of the supernatant,
containing small DNA fragments, was subjected to gel electrophoresis,
while the other half, as well as the pellet containing large pieces of
DNA and cell debris, was used for the diphenylamine (DPA) assay (see
below).
Gel electrophoresis.
One-half of the supernatants was
treated with an equal volume of absolute isopropyl alcohol and 0.5 M
NaCl to precipitate the DNA and stored at 
20°C overnight. After
centrifugation at 13,800 × g for 15 min, the pellet
was washed with 200 µl of 70% ethanol and allowed to dry at room
temperature. The DNA was resuspended in 12 µl of TE solution (10 mM
Tris-HCl, 1 mM EDTA [pH 7.4]-3 µl of loading buffer (50%
glycerol, 1× Tris-acetate-EDTA, 10% saturated bromophenol blue, 1%
xylene cyanol) at 37°C for 20 min and then electrophoresed on a 1.7%
agarose gel containing 0.71 µg of ethidium bromide per ml for 1 h. Gels were photographed by using UV transillumination.
DNA fragmentation assay.
The DPA reaction was performed by
the method of Paradones et al. (33). Perchloric acid (0.5 M)
was added to the pellets containing uncut DNA (resuspended with 200 µl of hypotonic lysis buffer) and to the other half of the
supernatants containing DNA fragments, and then 2 volumes of a solution
containing 0.088 M DPA, 98% (vol/vol) glacial acetic acid, 1.5%
(vol/vol) sulfuric acid, and 0.5% (vol/vol) 1.6% acetaldehyde
solution was added. The samples were stored at 4°C for 48 h. The
colorimetric reaction was quantitated spectrophotometrically at 575 nm,
using a model UV-160A UV spectrophotometer (Shimazu Co. Ltd., Tokyo,
Japan). The percentage of fragmentation was calculated as the ratio of DNA in the supernatants to the total DNA.
Flow cytometric analysis.
Nuclear DNA content was analyzed
by flow cytometry (Becton Dickinson, Pont de Claix, France) after
propidium iodide staining by the method described by Nicoletti et al.
(32). Cells were pelleted, resuspended in hypotonic
fluorochrome solution (50 µg of propidium iodide per ml in 0.1%
sodium citrate-0.1% Triton X-100), and kept at 4°C in the dark
overnight before the analysis.
Detection of morphological apoptosis.
After
treatment with reagents, cells were fixed with 2% glutaraldehyde
solution (TA AB Laboratory, Aldermastone, England) for 1 h and
stained with 0.2 mM Hoechst 33258 to visualize the location of
DNA. Cells were examined with a fluorescence microscope (BHT-RFC;
Olympus, Tokyo, Japan) for determination of fragmentation of nuclei
and/or condensation of chromatin.
Reagents.
Hoechst 33258 [2'-(4-hydroxyphenyl)-5-(4-methyl-1-piperazinyl)-2,5'-bi-1H-benzimidazole],
saturosporine, and EGTA were purchased from Sigma. H-7
[1-(5-isoquinolinesulfonyl)-2-methylpiperazine dihydrochloride] and
HA1004 (5-isoquinolinesulfonamide dihydrochloride) were from Seikagaku
Kogyo (Tokyo, Japan). Genistein (4',5,7-trihydroxyisoflavone) and
herbimycin A were from Wako Pure Chemical Co. (Osaka, Japan). W-7
[N-(6-aminohexyl)-5-chloro-1-naphthalenesulfonamide-HCl]
was from Funakoshi Co. (Tokyo, Japan).
Statistics.
The significance of differences between groups
was determined by Student's t test.
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RESULTS |
Effect of culture filtrates on DNA fragmentation.
After a 48-h
growth period, the pH of P. gingivalis, P. loescheii, P. intermedia, and F. nucleatum spent media regularly ranged from 6.5 to 6.8, while the
pH of A. actinomycetemcomitans and C. ochracea spent media regularly ranged from 6.0 to 6.3. The induction of apoptosis by culture filtrates was indicated by
the colorimetric DNA fragmentation assay. The spent media of
P. gingivalis, P. loescheii, and
F. nucleatum significantly increased the amount of DNA
fragmentation compared with the control media, BHI, for the bacterial
cultures in WEHI 231 cells (P < 0.01; Fig.
1). On the other hand, the supernatants
from P. intermedia, A. actinomycetemcomitans, and C. ochracea did not affect
DNA fragmentation. When we tested various dilutions of the bacterial
culture filtrate, it was possible to induce apoptosis if the
control levels were reduced to near zero with lower concentrations of
the filtrate of P. gingivalis, P. loescheii, and F. nucleatum. The level of
spontaneous apoptosis in WEHI 231 cells which are cultured only
in complete medium for 21 h was 9.8% ± 1.0%. Although in our
study a sterile BHI medium, after 21 h of culture, induced a
slight apoptosis, the number of induced apoptotic cells was
negligible compared to that seen after exposure of the cells to the
culture filtrate of P. gingivalis, P. loescheii, and F. nucleatum. However, this result
suggests that the trace amounts of apoptosis-inducing factor
present in this preparation may contribute to DNA fragmentation.
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FIG. 1.
Effect of spent medium from periodontopathic bacteria on
DNA fragmentation. WEHI 231 cells were cultured for 21 h with 100 µl of bacterial spent medium. Harvested cells were assayed by the DPA
assay. The results are expressed as the mean ± SE from three
different experiments with triplicate cultures. The level of
spontaneous apoptosis in WEHI 231 cells cultured only in
complete medium for 21 h was 9.8% ± 1.0%. Values significantly
different from those for the controls at P < 0.01 (**) are indicated.
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Effect of volatile fatty acids on cell proliferation.
We
examined the effects of various concentrations of volatile fatty acids
on the proliferative activity of mouse WEHI 231 cells and human RAJI
cells. After 21 h of incubation, the volatile fatty acids caused a
reduction in cell proliferative activity, as assessed by the
colorimetric MTT assay. WEHI 231 cells exhibited a marked,
dose-dependent response to butyric, propionic, and isovaleric acids
(Fig. 2A). With 5 mM butyric, propionic,
and isovaleric acids, the proliferative responses of WEHI 231 cells
were significantly suppressed by 84.5, 73.5, and 69.9%, respectively.
While butyric acid also exhibited a dose-dependent inhibition in RAJI
cells, propionic and isovaleric acids were less effective (Fig. 2B). The decrease of both cell proliferation by butyric acid prompted us to
determine the type of cell death induced by butyric acid.
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FIG. 2.
Dose-dependent effects of volatile fatty acids on cell
proliferation. WEHI 231 (A) and RAJI (B) cells were cultured with
butyric, propionic, and isovaleric acids for 21 h. Cellular
proliferation was determined by the MTT assay and expressed as
percentage of the absorbance value obtained without volatile fatty
acids. The results are expressed as the mean ± SE from three
different experiments with triplicate cultures.
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DNA fragmentation caused by butyric acid.
The induction of
apoptosis by butyric acid was indicated by the colorimetric DNA
fragmentation assay, electrophoresis of the fragmented DNA, nuclear
morphology, and flow cytometric analysis of DNA contents. When the
three types of B cells (WEHI 231, splenic B, and RAJI cells) were
cultured in the presence of 0.31 to 5.0 mM butyric acid for 21 h
and quantitated by the DNA fragmentation assay, a dose-dependent
increase in DNA fragmentation was seen (Fig.
3A). Butyric acid induced a substantial
and near-maximal (69.4% with 5 mM butyric acid) increase in DNA
fragmentation (62.6%) for WEHI 231 cells at 1.25 mM (P < 0.01). For splenic B cells and RAJI cells, 2.5 mM butyric acid
increased the amount of DNA fragmentation to 50.9 and 31.5%,
respectively (Fig. 3A). These results indicate that different degrees
of apoptosis induction by butyric acid depend on the
differences in sensitivity of the cell population. In similar
experiments, cells were cultured with 5 mM butyric acid and examined
for DNA fragmentation at various times over a 21-h time period (Fig.
3B). Treatment of WEHI 231 cells with butyric acid for 6 h
resulted in a markably increase in DNA fragmentation.
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FIG. 3.
Dose-response curves and time course of butyric
acid-induced apoptosis. (A) WEHI 231 ( ), RAJI ( ), and
splenic B ( ) cells were cultured with butyric acid for 21 h.
(B) WEHI 231 cells were cultured in the presence () or absence ()
of butyric acid (5 mM). Harvested cells were assayed by the DPA assay.
The results are expressed as the mean ± SE from three different
experiments with triplicate cultures. Values significantly different
from those for the controls at P < 0.01 (**) and
P < 0.05 (*) are indicated.
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The induction of apoptosis by butyric acid in the B-cell
population was further confirmed by electrophoresis of fragmented
DNA
(Fig.
4A). Low-molecular-weight DNA
fragments extracted from
WEHI 231 cells cultured with various
concentrations of butyric
acid for 16 h showed typical
oligonucleosomal ladders in a concentration-dependent
fashion (Fig.
4A). Negligible cleavage of DNA into nucleosomal
fragments was seen
with untreated WEHI 231 cells. When we examined
the morphological
changes in the nuclei of 5 mM butyric acid-treated
WEHI 231 cells by
DNA staining with Hoechst 33258, the characteristic
features of
apoptosis, including condensation and aggregation
of chromatin
near the nuclear membrane, were observed (Fig.
4B).
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FIG. 4.
(A) Agarose gel electrophoresis of DNA extracted from
WEHI 231 cells treated with butyric acid for 16 h. Lanes: M,
molecular weight markers (HaeIII-digested  X174 DNA); 1, untreated control cells; 2 to 6, cells treated with 5, 2.5, 1.25, 0.62, and 0.31 mM butyric acid. (B) Fluorescence microscopy appearance of
WEHI 231 cells untreated or treated with butyric acid for 16 h and
stained with Hoechst 33258. Normal nuclear morphology is observed in
untreated cells; in contrast, small and condensed nuclei with typical
apoptotic morphology are observed in treated cells.
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The DNA content of butyric acid-treated WEHI 231 cells, stained by
propidium iodide, was also analyzed with a flow cytometer
(Fig.
5). Apoptoic nuclei were
distinguishable by the hypodiploid
DNA contents compared with the
diploid DNA contents of normal
cells. A single peak of DNA,
indicating diploid DNA content, characterized
untreated WEHI 231 cells. In contrast, the percentage of WEHI
231 cells with hypodiploid
DNA was increased by treatment with
butyric acid in a
time-dependent fashion. Flow cytometric analysis
revealed that
DNA degradation appeared to occur 3 h after butyric
acid
treatment.
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FIG. 5.
Flow cytometric analysis of untreated (left) and 5 mM
butyric acid-treated (right) WEHI 231 cells. Cells were cultured for 1, 3, 7, and 16 h. DNA content was analyzed by propidium iodine
staining. Note the hypodiploid DNA peak typical of apoptosis in
treated cultures.
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Cell cycle distribution induced by butyric acid.
Flow
cytometric analysis of WEHI 231 cells treated with butyric acid
revealed that the cells were blocked at the G1/S interface of the cell cycle in time-dependent fashion (Table
1). By 7 h, control cells had
progressed through the cycle to more or less the same distribution as
at 1 h, whereas the butyric acid-treated cells showed both an
increase in G1 and a decrease in S and G2/M cells. This arrest of the suppressed cells in vitro was found to be
unresponsive to removal of butyric acid (data not shown). Furthermore,
in RAJI cells, 21-h treatment with 5 mM butyric acid also caused the
G1 phase arrest, after some delay compared to WEHI 231 cells (data not shown). These results suggest that butyric acid
blocks transition of the cells from G1 to the S phase of the cell cycle and the thereby irreversibly halts the progression of
WEHI 231 and RAJI cells to mitosis.
Effect of modulators of intracellular signal transduction
pathway.
To investigate the intracellular mechanism involved in
the induction of butyric acid-induced B-cell apoptosis, the
involvement of known intracellular signal transduction pathways was
examined by use of specific modulators of protein phosphorylation
systems and Ca2+ signaling (17, 20). As shown in
Fig. 6, protein kinase C inhibitors H-7
and staurosporine, tyrosine kinase inhibitors genistein and herbimycin
A, protein kinase A/G inhibitor HA1004, and extracellular Ca2+ chelator EGTA showed little or no apparent effect on
DNA fragmentation of butyric acid-treated WEHI 231 cells and splenic B
cells. On the other hand, among the modulators of Ca2+
signaling, W-7 significantly (P < 0.01) inhibited DNA
fragmentation of butyric acid-treated cells (57.8 to 25.2% for WEHI
231 cells and 53.5 to 17.9% for splenic B cells). W-7 also inhibited
DNA fragmentation of human Jurkat T cells and mouse thymocytes treated with butyric acid (data not shown). Chlorpromazine, another modulator of Ca2+ signaling, also inhibited DNA fragmentation of
butyric acid-treated WEHI 231 cells (data not shown). Since both W-7
and chlorpromazine have the ability to inhibit calmodulin function
(17), it is suggested that calmodulin participates in the
induction of butyric acid-induced apoptosis.
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FIG. 6.
Effects of various inhibitors on butyric acid-induced
apoptosis. WEHI 231 and splenic B cells were treated with
various inhibitors in the presence of 5 mM butyric acid for 21 h.
Harvested cells were assayed by the DPA assay. The results are
expressed as the mean ± SE from three different experiments with
triplicate cultures. Values significantly different from those for the
controls at P < 0.01 (**) are indicated.
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DISCUSSION |
The data presented here indicate that culture supernatant of
P. gingivalis, P. loescheii, and
F. nucleatum induced DNA fragmentation in WEHI 231 cells (Fig. 1). Since the volatile fatty acids found in the culture
filtrates consisted primarily of butyric and isovaleric acids for
P. gingivalis, propionic, butyric, and isovaleric acids for P. loescheii, and butyric acid for F. nucleatum, and these commercial volatile fatty acids significantly
depressed mouse splenic B-cell proliferation (23), we
hypothesized that volatile fatty acids in each culture filtrate have
B-cell apoptosis-inducing activity. In the present study, we
further demonstrated the capacity of volatile fatty acids, and butyric
acid in particular, to regulate proliferation and apoptosis of
B cells.
The data reported in this study indicate that different degrees of
inhibition of the human and mouse B-cell proliferative responses
resulted from exposure of the cells to the various volatile fatty acids
(Fig. 2). Especially butyric acid, which is a virulence factor common
to P. gingivalis, P. loescheii, and
F. nucleatum (23), suppressed 79.3 and
40.6% of WEHI 231 cells and RAJI cell proliferation, even at a low
concentration (1.25 mM). On the basis of our previous results showing
that 13.3 to 26.8 mM butyric acid was detected in culture filtrates
from the above three strains (23), along with a previous
study showing that butyric acid concentrations in subgingival plaque
from periodontitis sites could reach 14.4 to 20.0 mM (25,
30), and its concentration in periodontal pockets has been shown
to correlate with the severity of periodontal disease (4),
butyric acid can be recognized as an important virulent factor of these
periodontopathogens. On the other hand, a very low level (0.15 mM) of
propionic and isovaleric acids stimulated the proliferation of RAJI
cells (Fig. 2A), and the same level of butyric acid also mediated the
proliferation of human epithelial and fibroblast cell line (data not
shown). Tumor necrosis factor is cytotoxic to some tumor cells but
stimulates the proliferation of other cell types (2). Fas
signal transduction also triggers either proliferation or
apoptosis in human fibroblasts, depending the magnitude of Fas
expression (1, 14). Although it is not clear on what the
balance between cell proliferation and loss by death depends, our
results suggest that the signal induced by butyric acid must mediate
not only cytotoxic but also proliferative signals.
We have shown that in vitro, butyric acid-stimulated mouse WEHI 231 cells, splenic B cells, and human RAJI cells underwent apoptosis a specific form of programmed cell death
characterized by internucleosomal DNA digestion, revealed by
colorimetric DNA fragmentation assay (Fig. 3) followed by gel
electrophoresis (Fig. 4A). Cell death was also associated with
chromatin condensation (Fig. 4B) and flow cytometric determination of
the proportion of cells with hypodiploid DNA (Fig. 5).
Flow cytometric analysis revealed that maximal DNA degradation appeared
to occur 16 h after butyric acid treatment (Fig. 3B), as evidenced
by the maximal appearance of DNA with low fluorescence (Fig. 5).
Kinetic studies of flow cytometric cell cycle analysis of propidium
iodide-stained WEHI 231 cells treated with butyric acid revealed the
appearance of a "sub-G1" population below the G1 region. This extra sub-G1 peak displaying
reduced fluorescence of the DNA is likely due to a reduction in cell
volume and nuclear condensation characteristics of apoptoic cells
(9). Cell cycle distribution also changed during incubation:
after 7 h of incubation, butyric acid treatment resulted in fewer
cells in the S and G2/M phases of the cell cycle, which
means that butyric acid-induced inhibition of cell growth was
correlated to an arrest in the G1 phase of the cell cycle
(Table 1). These findings suggest that the proliferation inhibition and
apoptosis induction are dependent on G1-phase
accumulation. This G1-phase accumulation occurred prior to maximal DNA
fragmentation observed at 16 h, as shown in Fig. 3B. Our previous
study (24) showed that butyric acid arrested Jurkat cells at
the G1 phase. Furthermore, similar results demonstrated
that butyric acid induced a blockage in the G1 phase of the
cell cycle in a human colon cancer cell line (29) and in a
human myeloid leukemic cell line (6). These results suggest that G1 arrest due to butyric acid is a general property of
this agent.
Eukaryotic cell cycle progression is controlled by an evolutionarily
conserved mechanism, which requires the sequential activation of a
series of serine/threonine protein kinases, the cyclin-dependent kinases (Cdks) (13). Cell cycle regulation by extracellular signals such as growth factors is likely to take place primarily in the
G1 phase of the cell cycle, because cells become refractory to external signals once they are committed to replicate DNA
(34). Several lines of evidence suggest Cdk inhibitors play
an important role in growth regulation by external signals.
p21CIP1/SDI1/WAF1 is involved in irradiation-
and serum starvation-induced G1 arrest (11).
Moreover, p27kip1 has been shown to mediate cell
cycle arrest induced by cell-cell contact or transforming growth factor
in fibroblasts and epithelial cells (44) and that
induced by cyclic AMP in macrophages (22). Evidence also
suggests that p27kip1 is involved in the surface
immunoglobulin-mediated growth arrest and in the CD40-mediated cell
cycle progression of WEHI 231 cells (19). Therefore, it is
possible that Cdks and Cdk inhibitors play important roles in butyric
acid-induced cell proliferation and apoptosis. Further studies
will be required to clarify this possibility.
Interest in the action of butyrate was greatly increased since the
demonstration that the molecule exerts a potent differentiating and
antiproliferative effect. The molecule affects gene expression at
different levels (5), but few data are available on its intracellular targets. Recent report indicates that treatment of K562
cells with sodium butyrate increases tyrosine phosphorylation and
activation of mitogen-activated protein kinase (36).
Russo et al. (38) demonstrated that casein kinase II
down-regulation is involved in the signal transduction
pathway started by butyrate. Although some studies have shown that
inhibition of DNA synthesis by butyric sodium salt is associated with a
hyperacetylation of histones H3 and H4 due to an
n-butyrate-induced decrease in activity of some histone
deacetylase (3, 35), the mechanism of butyric acid-induced apoptosis is still unknown.
With respect to the mechanism by which butyric acid elicits
apoptosis, butyric acid triggers apoptosis by means of
calmodulin-dependent enzymes. Calcium and calmodulin have been
implicated as participants in various apoptoic signaling pathways.
Ionomycin, which allows Ca2+ entry into cells, increases
apoptosis in phorbol ester-treated T cells (28), and
glucocorticoid-induced T-cell apoptosis is associated with
calmodulin mRNA induction (10, 39). Although there is some
evidence that in some cells apoptoic degradation of DNA may occur via a
non-calcium-dependent endonuclease (26), the characteristic
DNA fragmentation process frequency depends on activation of a
Ca2+-dependent endogenous endonuclease (7), and
calmodulin inhibitors can reduce the activity of this
Ca2+-dependent endonuclease (27). Recently,
Cohen et al. (8) identified a novel cytoskeleton-associated
cell death serine/threonine kinase whose activation by
Ca2+/calmodulin may be linked to the biochemical mechanism
underlying the cytoskeletal alterations that occur during cell death.
Thus, calmodulin may play a direct role in regulating the enzyme
responsible for the characteristic extensive chromatin and DNA damage
of apoptosis.
In conclusion, we have reported here that culture filtrates of
periodontopathic bacteria and butyric acid present in the filtrate induce apoptosis in murine WEHI 231 cells, splenic B cells, and human RAJI cells. This specific form of programmed cell death was
characterized by DNA fragmentation assay, gel electrophoresis, chromatin condensation, and flow cytometric analysis. These data support the hypothesis that activation of apoptosis is at least one essential step in the butyric acid-induced immunosuppressive pathway and that butyric acid can modulate the immunoregulatory cell
population in periodontal tissue by inducing B-cell death through
apoptosis. We have tested other cell lines, including monocytes/macrophages, epithelial cells, and fibroblasts, but not T and
B cells, and demonstrated that butyric acid induced apoptosis
in monocytes/macrophages at similar levels as in T and B cells;
however, epithelial cells and fibroblasts were not as sensitive (data
not shown). Therefore, whatever the mechanism by which butyric acid
induces apoptosis, it is clear that a variety of cell lines are
susceptible. In fact, our data suggest that butyric acid may be an
apoptosis-inducing agent in most lymphoreticular cells.
| |
ACKNOWLEDGMENTS |
This work was supported in part by grants-in-aid (08672169) for
scientific research from the Ministry of Education, Science, and
Culture of Japan and by a Suzuki research grant from Nihon University
School of Dentistry at Matsudo.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Microbiology, Nihon University School of Dentistry at Matsudo,
Matsudo-shi, Chiba 271, Japan. Phone: 473-68-6111. Fax:
473-64-6295. E-mail: tkurita{at}mascat.nihon-u.ac.jp.
Editor: J. R. McGhee
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Abstract
Introduction
