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Infection and Immunity, December 2000, p. 6819-6825, Vol. 68, No. 12
Department of Medicine and Clinical
Science1 and Department of Cell
Pharmacology, Graduate School of Medicine,2 and
Physiological Chemistry, Faculty of Pharmaceutical
Sciences,3 Kyoto University, Sakyo, Kyoto, and
Physiological Chemistry, Asahikawa Medical University,
Asahikawa,4 Japan
Received 20 December 1999/Returned for modification 9 March
2000/Accepted 1 August 2000
In a previous study we showed that the involvement of EP4 subtype
of the prostaglandin E (PGE) receptor is crucial for lipopolysaccharide (LPS)-induced osteoclast formation in vitro. The present study was
undertaken to test whether EP4 is actually associated with LPS-induced
bone resorption in vivo. In wild-type (WT) mice, osteoclast formation
in vertebrae and tibiae increased 5 days after systemic LPS injection,
and urinary excretion of deoxypyridinoline, a sensitive marker for bone
resorption, statistically increased 10 days after injection. In EP4
knockout (KO) mice, however, LPS injection caused no significant
changes in these parameters throughout the experiment. LPS exposure for
4 h strongly induced osteoclast differentiation factor (ODF) mRNA
expression in primary osteoblastic cells (POB) both from WT and EP4 KO
mice, and this expression was not inhibited by indomethacin, suggesting
prostaglandin (PG) independence. LPS exposure for 24 h further
induced ODF expression in WT POB, but not in EP4 KO POB. Indomethacin
partially inhibited ODF expression in WT POB, but not in EP4 KO POB.
These data suggest that ODF is induced both PG dependently and PG
independently. LPS exposure for 24 h induced slightly greater
osteoclastgenesis inhibitory factor (OCIF) mRNA expression in EP4 KO
than in WT POB. These findings suggest that the reduced ODF expression
and apparently increased OCIF expression also are responsible for the
markedly reduced LPS-induced osteoclast formation in EP4 KO mice. Our
results show that the EP4 subtype of the PGE receptor is involved in
LPS-induced bone resorption in vivo also. Since LPS is considered to be
largely involved in bacterially induced bone loss, such as in
periodontitis and osteomyelitis, our study is expected to help broaden
our understanding of the pathophysiology of these conditions.
Osteomyelitis, bacterial arthritis,
and periodontal diseases are all caused by bacterial infection
(13, 24). Since bacteria do not invade the periodontal
tissues, the release of soluble bacterial factors is thought to be
involved in the pathogenesis of these forms of bacterially induced bone
destruction. Lipopolysaccharide (LPS) is the most likely candidate for
mediating these processes. LPS has been reported to potently stimulate
bone resorption in both in vitro and in vivo studies (12, 16,
26). LPS was reported to induce osteoclast formation in bone
marrow culture, and local injection of LPS into the femur was found to
lead to a rapid increase in the number of osteoclasts and the area of eroded surface. These findings indicate that increased osteoclast formation is involved in LPS-stimulated bone resorption. Osteoclast formation is an important step in bone resorption, since only osteoclasts can actively resorb bone and have a short life span, less
than 2 weeks (8, 23). Osteoclasts originate from
hematopoietic stem cells and belong to the monocyte/macrophage lineage
(36, 39). Differentiation into osteoclasts is influenced by
many systemic and local factors, such as hormones, cytokines, growth factors, and eicosanoids. LPS has been known to stimulate the production of many local factors, including tumor necrosis factor PGs, especially of the E series, are potent bone-active substances,
PGE2 was reported to potently resorb bone and enhance bone
formation both in vitro and in vivo (27, 29). Until
recently, however, the mechanism of action of PGs remained largely
unknown. Recently, though, PG receptors have been cloned and thoroughly characterized. Four PGE receptor subtypes have been cloned in mice.
They are coupled with different intracellular signaling mechanisms: EP1
with calcium mobilization, EP2 and EP4 with the stimulation of
adenylate cyclase, and EP3 mainly with the inhibition of adenylate
cyclase (10, 14, 18, 37, 42). On the basis of these recent
findings, we aimed to determine through which subtype of PGE receptor
each of the various skeletal actions of PGE2 is exerted.
We recently studied the mechanism of PGE2-induced
osteoclast formation in the coculture (30), and EP4 agonist
was found to be far more potent in osteoclast formation than any other
agonists. Therefore, we studied EP4 subtype-deficient (EP4 knockout
[KO]) mice, which have been recently generated by us, to clarify the importance of EP4 in bone. Most EP4 KO mice died shortly after birth
because of failure to close of the ductus arteriosus, a blood vessel
which bypasses pulmonary circulation during fetal life (25,
32). EP4 KO mice which survived to adulthood had no skeletal
abnormalities as seen by their gross appearance, soft X-ray analysis,
or histological examination. Since these results suggest that EP4 is
not essential for the bone function under the basal condition, we then
studied the role of EP4 under the disease state, where PGE2
production is increased. We first studied the involvement of the EP4
subtype in exogenously added PGE2-induced osteoclast
formation. Our data clearly showed that PGE2 enhances osteoclast formation through the EP4 subtype on primary osteoblastic cells (POB), not on osteoclast precursors. We then studied the possible
involvement of the EP4 subtype in osteoclast formation induced by
IL-1 In order to follow up on this evidence that the EP4 subtype of the PGE
receptor is crucially involved in LPS-induced osteoclast formation in
vitro, the aim of the study reported here was to test the in vivo
relevance of this finding.
Reagents.
LPS (Escherichia coli 0127:B8) was
purchased from Difco Laboratories (Detroit, Mich.). The osteoclast
differentiation factor (ODF) and osteoclast inhibitory factor
(OCIF) cDNAs were prepared by reverse transcription-PCR as previously
described (20, 45). Generation of EP4 KO mice.
Details of the generation of EP4
KO mice have been described elsewhere (25, 32). In brief, a
1.6-kb fragment containing the coding region from Asn-32 in the
N-terminal region to Val-317 in the sixth transmembrane region was
replaced with a neomycin resistance gene. The targeting vector was then
electroporated into E14-1 ES cells. Chimeric males were mated to
C57BL/6 females, and homozygous mutant mice were obtained by
interbreeding of heterozygous mice.
Treatment.
Each experiment included the WT and EP4 KO
groups, consisting of seven mice each. The mice were male, 11 weeks
old, weighed approximately 25 g, and were age matched. There was
no significant difference in body weight between WT and EP4 KO mice.
LPS (20 mg/kg of body weight) diluted on sterile 0.01 M
phosphate-buffered saline (PBS) or PBS was injected subcutaneously into
the back of WT mice or EP4 KO mice (1). Urine was collected
before and on days 5, 7, 10, and 14 after injection. Urinary excretion
of deoxypyridinoline (D-Pyr) was measured with an enzyme immunoassay kit (Pyrilinks-D; Metra Biosystems Inc., Mountain View, Calif.) and was
corrected by simultaneously measured urinary creatinine concentration
(40). Serum was collected before and on days 3, 5, 7, 10, and 14 after injection. Serum osteocalcin levels were measured with a
radioimmunoassay kit (mouse osteocalcin RIA reagents; Biomedical
Technologies Inc., Stoughton, Mass.).
Histomorphometry.
Vertebrae (lumbar 2 to 4) and tibiae from
WT and EP4 KO mice were prepared before and on days 5 and 10 after LPS
injection. The vertebrae and tibiae were fixed in 4%
paraformaldehyde-PBS (pH 7.2) for 24 h, decalcified by means of
10% EDTA-PBS (pH 7.2) for 7 days, dehydrated in a graded
concentration of ethanol, and embedded in paraffin according to the
standard procedure. Five-micrometer-thick sections were placed on
APS-coated glass slides (Matsunami, Osaka, Japan) and stained for
tartrate-resistant acid phosphate (TRAP) using a naphthol ASTR (Sigma
Chemical Co., St. Louis, Mo.) (9). For each lumbar vertebra
and tibia, two rectangular areas of interest with a width of 0.45 mm
were randomly assigned for analysis, extending 0.2 to 0.4 mm from the
growth plate. For each group of seven mice, the results were averaged.
Osteoclasts were identified as TRAP-positive cells when they had three
or more nuclei, directly faced a bone surface, or were located in a
resorption cavity.
Cell culture, RNA extraction, and Northern blot analysis.
POB were isolated from the calvariae of 1-day-old WT and EP4 KO mice by
sequential digestion with bacterial collagenase and dispase
(34). POB (3.5 × 103
cells/cm2) from WT mice and EP4 KO mice were seeded in
6-cm-diameter plates, and cultured in Statistical analysis.
To test statistical significance
between two groups, Student's t test was used. For more
than two groups, an analysis of variance was used to determine which
groups were significantly different. A P value of <0.05 was
considered to be statistically significant.
Urinary excretion of D-Pyr.
Systemic LPS injection into WT
mice caused a statistically significant increase in the urinary
excretion of D-Pyr, which is a sensitive marker for bone resorption. It
was approximately 140% of the initial value on day 10 and
approximately 160% on day 14 in WT mice (Fig.
1). In contrast, there was no significant
increase of D-Pyr in EP4 KO mice throughout the experiment (day 0 through 14) (Fig. 1).
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Impaired Bone Resorption by Lipopolysaccharide In
Vivo in Mice Deficient in the Prostaglandin E Receptor EP4
Subtype
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
(TNF-), interleukin-1 (IL-1), and prostaglandin E2
(PGE2) from macrophages, fibroblasts, and osteoblastic
cells in inflamed periodontal tissues (2, 3, 24). Despite
rigorous studies by many researchers (4, 5, 11, 22, 46),
however, the molecular mechanism of LPS-induced osteoclast formation
remains unknown. We therefore focused our attention on the involvement
of prostaglandin (PG) in LPS-induced osteoclast formation, based on the
recently cloned PG receptor and the results of our recent studies on
the skeletal action of PGs (see below).
, TNF-, basic fibroblast growth factor (bFGF), and LPS. All
these molecules markedly enhanced osteoclast formation in the coculture
from wild-type (WT) mice but not in the coculture from EP4 KO mice.
Furthermore, they significantly induced prostaglandin G/H synthase-2
(PGHS-2) (which is the inducible form of the rate-limiting enzyme in PG
synthesis) mRNA expression in POB, and osteoclast formation by these
molecules was almost completely eliminated by the PGHS inhibitor
indomethacin. Therefore, the likely mechanism of osteoclast formation
by IL-1, TNF-, bFGF, and LPS is that they increase PG production
by inducing PGHS-2 in POB and that PGE2, in turn,
stimulates osteoclast formation mainly via the EP4 subtype on osteoblasts.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-Actin cDNA probe and indomethacin
were purchased from Wako Chemical Industry (Tokyo, Japan).
-minimum Eagle's medium
containing 10% fetal bovine serum (JRH Biosciences, Lenexa, Kans.). At
confluency, cells were cultured in a starvation medium (-minimum
Eagle's medium containing 0.1% fetal bovine serum) for 24 h and
exposed to LPS (100 ng/ml) with or without indomethacin
(10
7 M). After a 4- or 24-h incubation, total RNA was
extracted with an RNA Easy Kit (QIAGEN). The RNA was then
electrophoresed on a 1.2% agarose gel and transferred onto a Biodyne B
membrane (Pall Biosupport, East Hills, N.Y.) and hybridized with ODF,
OCIF, and -actin probes labeled with [-32P]dCTP.
Hybridization was carried out at 42°C overnight in a hybridization buffer (50% deionized formamide, 5× SSC [1× SSC is 0.15 M NaCl plus
0.015 M sodium citrate], 5× Denhardt's solution, 0.2% sodium dodecyl sulfate [SDS], 200 µg of sonicated salmon sperm DNA per ml). The membrane was washed with a washing buffer (2× SSC-0.1% SDS
and 0.2× SSC-0.1% SDS), and the radioactivity was analyzed by a
bioimage analyzer (BAS 2000; Fuji Film, Tokyo, Japan). The levels of
ODF and OCIF mRNAs were analyzed relative to that of -actin.
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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FIG. 1.
Effect of systemic LPS injection on urinary excretion of
D-Pyr. LPS (20 mg/kg of body weight) was injected subcutaneously into
11-week-old WT mice or EP4 KO mice. The ratios of D-Pyr (nanomolar)
creatinine (Cr) (millimolar) before injection (day 0) and on days 5, 7, 10, and 14 after injection are shown. Values for the basal level
(before injection) were assigned 100% in each case. Data are expressed
as the mean + standard deviation (error bar). (n = 7). *, P < 0.05.
Histomorphometric analysis of lumbar vertebrae and tibiae.
Osteoclast formation was evaluated by counting the number of cells
which were positively stained with TRAP. After systemic injection of
LPS into the WT mice, the number of osteoclasts of the lumbar vertebrae
statistically significantly increased to approximately 150% of the
basal level on day 5 and returned to almost the basal level on day 10. In sharp contrast, LPS injection into the EP4 KO mice caused no
significant increase in the number of osteoclasts throughout the
experiment (Fig. 2).
|
Serum osteocalcin levels.
After systemic injection of LPS,
serum osteocalcin levels had decreased to approximately 40% of the
basal level by day 3 after injection and returned to the initial values
10 days after injection. Throughout the experiment, there was no
significant difference between WT and EP4 KO mice (Fig.
3).
|
ODF and OCIF mRNA expressions in POB.
ODF mRNA expression was
hardly detectable under the basal condition (after 24 h of
starvation) in POB from either WT or EP4 KO POB. LPS (100 ng/ml)
exposure for 4 and 24 h markedly and time dependently induced ODF
mRNA expression in POB from WT mice. In POB from EP4 KO mice, LPS
exposure for 4 h induced ODF mRNA at almost the same level as WT,
and LPS exposure for 24 h increased ODF expression, though this
increase was minimal (Fig. 4A).
|
-actin induced by LPS exposure for
4 h was approximately 15 times the basal level (average of four
independent experiments) in POB from WT and EP4 KO mice. The ODF level
induced by LPS exposure for 24 h was 240% ± 43% (from four
independent experiments) of that induced by LPS exposure for 4 h
in POB from WT mice. In contrast, the ODF level induced by LPS exposure
for 24 h was 118% ± 24% of that induced by LPS exposure for
4 h in EP4 KO mice, which was significantly lower than that in WT
mice (Fig. 4B). The ODF level induced by LPS exposure for 4 h was
not inhibited by indomethacin either in WT or EP4 KO POB. In contrast,
the ODF level by LPS exposure for 24 h was inhibited 34% ± 15%
by indomethacin in WT POB, but it was not inhibited by indomethacin in
EP4 KO POB.
OCIF mRNA expression was not significantly different under the basal
condition between POB from WT and that from EP4 KO mice. LPS (100 ng/ml) exposure for 4 h caused no appreciable changes in OCIF mRNA
expression in POB from either WT or EP4 KO mice. LPS exposure for
24 h, however, increased OCIF mRNA expression in POB from both WT
and EP4 KO mice (Fig. 4A). OCIF levels normalized to -actin induced
by LPS exposure for 24 h were approximately 150% ± 27% of the
basal level in WT mice and 215% ± 49% of the basal level in EP4 KO
mice (average of four independent experiments) (Fig. 4B). OCIF levels
induced by LPS exposure were not affected by indomethacin, irrespective
of the cell origin (WT or EP4 KO), or duration (4 or 24 h).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Some studies have suggested the involvement of PGE2 in
LPS-induced bone resorption (15, 31). Inhibition of
LPS-induced bone resorption by inhibitors of PG synthesis has been
reported by several investigations. LPS was found to increase
45Ca release, hence bone resorption, from neonatal mouse
calvariae, and this increase was partly inhibited by indomethacin. More
specifically, the involvement of PG in LPS-induced osteoclast formation
has also been suggested. For example, Ueda et al. showed that
indomethacin inhibited LPS-induced osteoclast formation in bone marrow
cultures (41). Elevation of the number of osteoclasts after
LPS injection was reduced by about 50% by indomethacin
(107 M) in mouse calvariae (46). Furthermore,
flurbiprofen, a nonsteroidal anti-inflammatory drug and PGHS inhibitor,
reduced the alveolar bone loss associated with periodontitis in beagles
in vivo (43). In addition, Plotquin et al. reported that
PGE2 production was 5 to 30 times higher in osteomyelitic
human bones compared with control bones, whereas prostacyclin
production remained the same in these two types of bones
(28). These reports indicate that it is likely that
PGE2 at least partially mediates LPS-induced bone
resorption. However, these findings constitute indirect evidence and do
not provide information on the action mechanism of PGE2. To
follow up on our recent observation that the involvement of the EP4
subtype of the PGE receptor is essential for LPS-induced osteoclast
formation in vitro (30), the aim of the study reported here
was to determine whether this mechanism also functions in vivo. For
this purpose, LPS was injected systemically into WT and EP4 KO mice.
The overall bone resorption was evaluated by urinary excretion of D-Pyr. D-Pyr is a degradation product of the cross-link structure of triple helical type I collagen and is a very sensitive marker for bone resorption (40). LPS injection resulted in a marked increase in urinary D-Pyr excretion in WT but not in EP4 KO mice. Since these data suggest that the EP4 subtype of the PGE receptor is essential for LPS-induced bone resorption in vivo, we then studied whether the EP4 subtype is involved in LPS-induced osteoclast formation in vivo. Histological sections of the lumbar vertebrae and tibiae were stained for TRAP, which is a representative marker for osteoclasts. Histomorphometric analysis revealed that systemic injection of LPS significantly increased the number of osteoclasts of WT vertebrae and tibiae. Interestingly, on day 10 after LPS injection, osteoclast numbers in vertebrae returned to the basal level, in contrast, osteoclast numbers in tibiae remained increased. These results suggest that LPS produces generalized increases in osteoclasts, although each bone may respond to LPS with different time courses. In contrast, LPS caused little changes in osteoclast numbers in vertebrae or tibiae of EP4 KO mice. These results clearly show that the EP4 subtype is involved in LPS-induced osteoclast formation and bone resorption in vivo.
Our results indicated that the number of osteoclasts statistically increased 5 days after LPS injection but that the increase in urinary D-Pyr excretion did not become obvious until day 10 and had only slightly increased by day 7. A recent report also showed that the peak of osteoclast formation and of the area of the eroded surface covered by osteoclasts occurred on day 5 after LPS injection (9). At present, there is no clear explanation for this apparent discrepancy in the time course of the number of osteoclasts and urinary D-Pyr excretion. Although D-Pyr has not been studied in LPS-injected mice, similar findings have been reported in an ovariectomy model, with recent reports (7, 21) showing that deterioration in the trabecular bone connectivity and volume already occurred on day 5 after ovariectomy, while urinary D-Pyr excretion increased more slowly (on day 13). Probably some period is required before D-Pyr excretion increases, which reflects an increase in bone resorption by newly formed osteoclasts. Of further interest is the reduction in serum osteocalcin levels in both WT and EP4 KO mice after LPS injection. Since osteocalcin is a differentiation marker of osteoblasts, and hence of bone formation, these results suggest that LPS negatively affects bone formation both in WT and EP4 KO mice. Recently, LPS was reported to inhibit osteoblastic cell differentiation in rat calvarial cells (17). Although further studies are required, these data suggest that the EP4 subtype is involved in LPS-induced bone resorption but not in the negative influence of LPS on bone formation.
We subsequently studied the downstream mechanism of EP4. Osteoclast
formation is known to be enhanced by three major classes of stimuli:
the 1,25(OH)2 vitamin D3 pathway, the cyclic
AMP-mediated pathway (parathyroid hormone and PGE2), and
the gp-130 mediated pathway (IL-6, IL-11, and oncostatin M). Suda et
al. postulated that these molecules commonly induce a putative factor
to enhance osteoclast formation on osteoblasts (35).
Recently this putative common factor, the ODF (also known as
osteoprotegerin ligand, OPGL, RANKLE, or TRANCE) was cloned by several
groups of researchers. ODF is a TNF--like molecule, is induced on
the osteoblast plasma membrane by the stimuli mentioned earlier, and
enhances osteoclast differentiation through the interaction with its
receptor on osteoclast precursor cells (20, 38, 45). Another
molecule involved in this cell-cell interaction was cloned: the OCIF
(also known as osteoprotegerin or OPG). OCIF functions as a decoy
receptor and interferes with the interaction of ODF and its receptor
(33, 44). Their functional relevance is clearly shown by the
finding that ODF KO mice develop osteopetrosis and OCIF KO mice develop severe osteoporosis (6, 19). In the present study, LPS
exposure for 4 h strongly induced ODF mRNA expression in POB from
WT mice and EP4 KO mice. ODF levels in WT and EP4 KO were almost the
same, and this may be due to a PG-independent pathway, because the
levels were not inhibited by indomethacin. LPS exposure for 24 h
further increased ODF mRNA expression level (240% of that by LPS
exposure for 4 h) in WT POB, and this induction was inhibited
about 34% by indomethacin. These results suggest that ODF induction
was induced by not only a PG-dependent pathway but also a
PG-independent pathway such as a direct effect of LPS. Although LPS
exposure for 24 h increased ODF mRNA expression in EP4 KO mice
(118% of that by LPS exposure for 4 h), this increase was
minimal, and this induction was not inhibited by indomethacin. From
these results, a small increase in ODF expression in EP4 KO POB is
likely to be due to a PG-independent pathway rather than a PG-dependent pathway via another receptor except EP4 subtype. LPS induced slightly more OCIF mRNA expression in POB from EP4 KO mice than WT mice. These
findings suggest that the reduced ODF expression and apparently increased OCIF expression also are responsible for the aforementioned finding that bone resorption induced by LPS is markedly reduced in EP4
KO mice.
Our previous in vitro data showed, in the coculture using cells from
EP4 KO mice, little osteoclast was formed by PGE2, IL-1, TNF-, bFGF, and LPS, which suggests that osteoclast formation by
these molecules is mostly PG dependent. In contrast, osteoclast formation by 1,25(OH)2 vitamin D3 and
parthyroid hormone in the coculture from EP4 KO mice was only partially
decreased, which suggests that osteoclast formation by
1,25(OH)2 vitamin D3 and parathyroid hormone is
largely PG independent. The above findings, together with the current
data, suggest that impaired LPS-induced osteoclast formation is a
specific phenomenon in EP4 KO mice and not the nonspecific or indirect
consequence of the lack of EP4 receptor.
In conclusion, the involvement of the EP4 subtype of the PGE receptor is important for LPS-induced bone resorption in vivo. Antagonizing EP4 action may thus prove to be clinically useful for the treatment of bacterially induced bone loss, such as in periodontitis and osteomyelitis.
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ACKNOWLEDGMENTS |
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This work was supported by a grant-in-aid from the Ministry of Sciences, Education, and Culture and grants from the Research Association for the Metabolic Bone Diseases and the Smoking Research Foundation.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Medicine and Clinical Science, Graduate School of Medicine, Kyoto University, 54, Shogoin-kawaharacho, Sakyo, Kyoto 606-8507, Japan. Phone: 81-75-753-7509. Fax: 81-75-771-9452. E-mail: ktanaka{at}koshien.ac.jp.
Editor: R. N. Moore
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Discussion
References
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