(Received for publication, February 27, 1997, and in revised form, May 20, 1997)
From the Departments of Medicine, § Cell
Biology and Physiology, ¶ Biology, and the ** George M. O'Brien
Center for Kidney and Urological Diseases, Washington University School
of Medicine, St. Louis, Missouri 63110 and the
Department of
Biochemistry, Albany Medical College, Albany, New York 12208
Osteoclasts form an acidic compartment at their attachment site in which bone demineralization and matrix degradation occur. Although both the cysteine proteinases and neutral collagenases participate in bone resorption, their roles have remained unclear. Here we show that interstitial collagenase has an essential role in initiating bone resorption, distinct from that of the cysteine proteinases. Treatment of osteoclasts with cysteine proteinase inhibitors did not affect the number of resorption lacunae ("pits") formed on the surface of dentine slices, but it generated abnormal pits that were demineralized but filled with undegraded matrix. Treatment with metalloproteinase inhibitors did not alter the qualitative features of lacunae, but it greatly reduced the number of pits and surface area resorbed. Treatment of bone cells with an inhibitory anti-rat interstitial collagenase antiserum reduced bone resorption markedly. In the presence of collagenase inhibitors, resorption was restored by pretreatment of dentine slices with rat interstitial collagenase or by precoating the dentine slices with collagenase-derived gelatin peptides or heat-gelatinized collagen. Immunostaining revealed that interstitial collagenase is produced at high levels by stromal cells and osteoblasts adjacent to osteoclasts. These results indicate that interstitial collagenase can function as a "coupling factor," allowing osteoblasts to initiate bone resorption by generating collagen fragments that activate osteoclasts.
Normal bone turnover is highly regulated. Osteoclasts, the cells that degrade bone, require activation to trigger their bone-resorptive capacity. Once activated, osteoclasts secrete both protons and proteinases at their attachment site, resulting in dissolution of bone mineral and degradation of the matrix (1). Osteoclasts produce several cysteine proteinases (2-4), enzymes with acidic pH optima, of which cathepsin K appears to be essential for normal bone resorption (5, 6). Studies indicate that the major function of secreted cysteine proteinases is matrix degradation (3, 7).
The role of neutral metalloproteinases, a second class of proteinase produced in bone tissue (3, 8), is less clear. Members of the metalloproteinase family have neutral pH optima, are secreted as proenzymes, and contain a zinc atom at the active site (9, 10). Although some prior studies suggested that neutral metalloproteinases contribute to osteoclast matrix degradation (11), recent evidence indicates that osteoclasts do not produce collagenase (12). Collagenase is produced by cells of osteoblastic lineage and may be required for resorption of intact bone tissue (13-16). Observations that isolated osteoclasts that had no detectable collagenase activity were able to resorb bone prompted the suggestion that collagenase promotes resorption by removing unmineralized matrix from the bone surface, facilitating osteoclast attachment (8, 17, 18).
In this study we have examined the qualitative and quantitative roles of acid cysteine proteinases and interstitial collagenase in bone resorption by mouse marrow osteoclasts on dentine wafers. We demonstrate distinct roles for the two classes of enzymes and show that collagen degradation by interstitial collagenase produces collagen fragments that activate osteoclast bone resorption.
Reagents were supplied from Sigma unless noted
otherwise. SC444631 was
supplied by the Monsanto Corporation (St. Louis). 1,25-Dihydroxyvitamin D3 a generous gift from Dr. M. Uskokovi
(Hoffman-LaRoche; Nutley, NJ). Sperm whale teeth were obtained from the
U. S. Department of Marine Fisheries.
Marrow was flushed from
mouse long bones and cultured on tissue culture plates (5 × 107 cells/plate) in MEM D10 (
MEM with 10% FBS) with
10
8 M 1,25-dihydroxyvitamin D3
(OC medium) as described (19). On day 6 adherent cells, which included
many osteoclasts, as well as other cells, were scraped and replated in
OC medium on 1-cm2 sperm whale dentine slices in 24-well
plates. Cultures were incubated on dentine slices from day 6 to day 10 with or without proteinase inhibitors (25 µM E64, 10 µM SC44463, 10 µM eglin C). Cells were then
removed with 2% SDS and the bone slices prepared for scanning electron
microscopy (scanning EM) as described (19). Surface area resorbed was
quantified from a grid of 50-µM squares placed over
photographs of three random fields taken with no tilt angle from at
least three bone slices; grid intersections over pits were counted and
expressed as a percentage of total intersections.
In experiments testing whether acid cysteine proteinase activity was
required to remove matrix proteins from resorption lacunae, dentine
slices were biotinylated with 1.8 mM sulfosuccinimidyl 6-(biotinamido) hexanoate (Pierce) for 1 h at 22 °C in
phosphate-buffered saline, pH 7.0; the slice was then washed thoroughly
with MEM D10. Cross-sections of the biotinylated slices stained with
fluoresceinated avidin and examined by confocal microscopy showed that
the biotin penetrated only ~1 µm into the dentine slice (not
shown). Biotinylation of the dentine surface also did not significantly
alter osteoclast resorptive activity (not shown). After overnight
incubation of the biotinylated wafers in
MEM D10, marrow cultures
were plated as above ± 25 µM E64 and incubated for
5 days. The slices were then stripped of cells with 0.1 M
NaOH for 15 min, washed three times with HENAC (30 mM
HEPES, pH 7.4, 100 mM NaCl, 2 mM
CaCl2), blocked with HENAC plus FBS, and incubated with
streptavidin-coated latex beads (250-nm diameter; Sigma) diluted 1:100
in HENAC plus FBS. The slices were washed three times with
phosphate-buffered saline at either pH 5.0 or 7.4 and then incubated
with cathepsin B (Athens Research, Athens, GA; 250 µg/ml in
phosphate-buffered saline) at 37 °C for 12 h at either pH 7.4 or 5.0. The slices were then prepared for scanning EM and assayed as
above.
In studies testing the effect of anti-rat interstitial collagenase (rIC) antibody or preincubation with collagenase on resorption pit formation, marrow cells cultured in plates for 5 days were scraped and plated on dentine slices with either preimmune serum (1:50) or anti-rIC antiserum (1:50-1:500) in the medium. In the collagenase preincubation experiment, dentine slices were incubated for 12 h at 37 °C with 250 µg/ml rIC activated as described (20). In all experiments, fresh medium and antisera were added after 3 days, and slices were assayed for resorption pit formation after 5 days.
For experiments examining the effect of collagenase treatment on osteoclast adherence, marrow cultures were incubated overnight on 1-cm2 dentine slices ± metalloproteinase inhibitor SC44463 (25 µM). Slices were fixed with 2.5% glutaraldehyde, stained for tartrate-resistant acid phosphatase-positive (19), and the number of tartrate-resistant acid phosphatase-positive mononuclear, multinucleated, and giant cells/slice were counted (19).
For testing the effect of precoating dentine slices with collagen
fragments or heat-denatured collagen on bone resorption, type I
collagen from rat tendon (21) was gelatinized by incubation at 1.6 mg/ml in 0.4 M NaCl for 15 min at 60 °C. 1.6 mg/ml of
the denatured collagen was incubated with 7.5 µg/ml rIC for 90 min at
37 °C; slices were then incubated with 1.6 mg/ml of the either the
heat-denatured gelatin or proteolyzed gelatin for 3 h at 37 °C. The slices were washed and incubated overnight with MEM D10 at 37 °C. Mouse marrow cultured for 5 days on plates in OC medium was
scraped and applied to the slices ± SC44463 (25 µM)
as indicated, and resorption pit formation was assayed after 5 days.
Mouse marrow was cultured for 5 days on plates, scraped, and applied to biotinylated dentine slices ± 25 µM E64 (6 slices/treatment). After 5 days, slices were stripped of cells, labeled with streptavidin-coated latex beads, and digested with cathepsin B as described above. Beads released by proteolysis were collected by washing slices with a stream of phosphate-buffered saline (10 ml/slice) and centrifuging the bead-containing solution for 10 min at 10,000 × g. Beads from the control and E64-treated slices were resuspended in 30 µl of SDS-polyacrylamide gel electrophoresis sample buffer (22) and boiled for 10 min; the supernatant was separated by SDS-polyacrylamide gel electrophoresis on 15% gels, transferred electrophoretically to nitrocellulose (Schleicher & Schuell), and probed with an anti-collagen(I) antibody (Monsanto).
Immunocytochemistry and HistochemistryMouse marrow cultures on dentine slices were fixed with 2% formaldehyde in HENAC for 30 min, washed, permeabilized with 0.1% Triton X-100 in HENAC for 15 min, washed, and incubated overnight with HENAC plus 10% FBS and 5 mM sodium azide at 4 °C. Slices were then incubated with anti-H+-ATPase monoclonal antibody E11 (64 µg/ml) (23), and either rabbit interstitial collagenase serum or preimmune serum (both at 1:1,000 dilution) in HENAC with 10% FBS for 2 h at 22 °C. Slices were washed in HENAC with 10% FBS and incubated for 1 h with Texas Red-conjugated anti-mouse IgG and fluorescein-conjugated anti-rabbit IgG (Jackson Immunoresearch Laboratories, West Park, PA), both diluted 1:500 in HENAC with 10% FBS. After an overnight wash, the slices were photographed by phase-contrast and fluorescent microscopy; the location of each photograph was recorded, and the slices were then stained for tartrate-resistant acid phosphatase and alkaline phosphatase activity with commercial kits (Sigma), following the manufacturer's protocol.
Mouse bone marrow cells cultured for 5 days in the presence of
1,25-dihydroxyvitamin D3 generate osteoclasts in
vitro (24) and form resorption lacunae on sperm whale dentine
wafers in a reproducible manner that can be assessed qualitatively and
quantitatively by scanning EM (19). The effect on bone resorption of
several proteinase inhibitors was examined in this system (Fig.
1). The matrix metalloproteinases (MMPs)
are inhibited by tissue-derived inhibitors (TIMPs) and specific
peptidomimetic hydroxamates that bind to zinc complexed at the
catalytic site of the enzyme (25). Treatment of the marrow cultures
with the peptidomimetic hydroxamate inhibitor
SC444632 markedly decreased
the number of resorption pits formed and the surface area (Fig. 1). In
one experiment, the addition of 3.6 µM TIMP-1
(Ki ~109 M), purified as
described (28), also diminished both the number of resorption pits
formed and surface area resorbed (not shown). In contrast, the cysteine
proteinase inhibitors (29) E64 and leupeptin (not shown) did not
affect significantly the number or surface area of resorption pits
formed on the dentine slices (Fig. 1), nor did the serine
proteinase inhibitor eglin C (30); the inhibition of resorption pit
number was observed only with the metalloproteinase inhibitors.
Resorption pits formed in the presence of the metalloproteinase inhibitor appeared normal but were decreased in number (Fig. 1C, right panel). Pits formed in the presence of E64, however, were abnormal, with a shallow and "fuzzy" appearance (Fig. 1B, right panel); identical results were obtained with 25 µM leupeptin (data not shown). To determine whether the abnormal appearance was the result of undegraded matrix remaining in the pit, we biotinylated dentine slices3; analysis of the slices by fluorescent confocal microscopy indicated that the biotin label only penetrated about 1 µM into the dentine slice, whereas normal pits range in depth from 2 to 10 µM. The biotin-labeled dentine slices were incubated with marrow cells in the presence or absence of E64 for 5 days, and cells were removed with 0.1 M NaOH. 250 nm streptavidin-conjugated latex beads were allowed to bind to the slices, and the slices from the E64-treated cultures were then incubated with cathepsin B either at pH 7.4 or 5.0.
In controls (Fig. 2, A and
B), streptavidin-coated beads were found on the surface of
the dentine slice, but few were found within pits, whose depth exceeded
the 1-µm thickness of the biotin labeling. In the E64-treated
cultures, with cathepsin post-treatment at pH 7.4 (at which cathepsin B
is inactive), beads were abundant both on the undisturbed bone surface
and within pits (Fig. 2, C and D), indicating
that in the presence of E64, even the surface protein matrix of the
bone is not removed efficiently. Slices from E64-treated cultures that
were post-treated with cathepsin at pH 5 also had shallow pits, but few
beads were present within the pits (Fig. 2, E and
F). Fig. 2G provides a quantitative analysis of
these observations. The increase in bead density over pits in the
E64-treated cultures likely reflects increased access of the beads to
the biotin moieties in the demineralized matrix. To confirm that the
cathepsin was removing beads by proteolysis of the dentine matrix, we
collected beads after proteolysis from six slices from E64-treated
cultures versus six slices from control cultures and
analyzed them for collagen fragments by immunoblotting with an
anti-collagen antibody. Numerous collagen digestion products were
detected associated with beads from the slices from the E64-treated cultures, compared with relatively low levels of collagen fragments obtained from the control slices (Fig. 2H). In
summary, the results from Figs. 1 and 2 indicate that the cysteine
proteinases are required to degrade the matrix in resorption lacunae
and that the neutral metalloproteinases, in contrast, function in the
initiation of resorption lacuna formation.
Of the known neutral matrix metalloproteinases, interstitial
collagenase has been reported to be produced by rodent osteoblasts under certain conditions (13, 15, 31-33) and has been found associated
with bone matrix proteins and possibly osteoclasts (11). To determine
if interstitial collagenase was the metalloproteinase involved in
initiating bone resorption, we treated the marrow cultures with a
rabbit antiserum specific for rodent collagenase (anti-rIC; 34), which
inhibits its enzymatic activity (34, 35). Anti-rIC antiserum inhibited
resorption by the marrow cultures in a
concentration-dependent manner, with maximal inhibition
comparable to that of peptidomimetic hydroxamates (Fig.
3A, inset). In cultures treated with anti-rIC, the initiation of bone resorption was restored by pretreatment of dentine slices with rIC (Fig. 3A). These
results indicate that interstitial collagenase is the major
metalloproteinase involved in initiating bone resorption in mouse
marrow cultures.
It has been proposed that collagenase could promote bone resorption by enhancing osteoclast attachment to the bone surface (8, 17, 18). We found, however, that the number of attached osteoclasts in cultures treated with metalloproteinase inhibitors was no different from controls (Fig. 3B). Alternatively, collagenase could promote bone resorption by generating fragments of collagen which activate osteoclasts directly. To address this possibility, we examined the effect on resorption pit formation of treating dentine slices with gelatin predigested in vitro by rIC. As shown in Fig. 3C, treatment of marrow cultures with SC44463 inhibited resorption pit formation, as demonstrated above, but incubation of the bone slices with gelatin fragments generated by in vitro digestion with purified interstitial collagenase restored resorption activity to levels greater than or equal to control levels in the continued presence of SC44463. These results indicate that interstitial collagenase can initiate bone resorption by generating gelatin fragments that activate osteoclasts, rather than by clearing the bone surface of collagen.
Collagenase cleavage of collagen could be producing an activation signal either by generating a specific peptide as a cleavage product or by lowering the melting temperature of the collagen helix (9), allowing it to expose an activation signal concealed in the helical conformation. We found that heat-denatured gelatin was nearly as efficient as collagenase-cleaved gelatin at restoring bone resorption in collagenase-inhibited mouse marrow cultures (Fig. 3C), providing strong evidence in support of the latter mechanism.
Antiserum to interstitial collagenase was used to examine the
immunocytochemical distribution of the enzyme in the marrow cultures on
bone slices. Collagenase was not detected in osteoclasts but was found
at high levels in small cells having a fibroblast-like appearance, some
of which costained for alkaline phosphatase, a marker for osteoblasts
(Fig. 4). Cells that stained with the collagenase antibody were often observed surrounding resorptive osteoclasts, suggesting the possibility that they might be engaged in
initiating bone resorption. These findings do not eliminate the
possibility that osteoclasts also produce interstitial collagenase; but
if they do, it must be present at low levels compared with the
surrounding stromal cells.
This study demonstrates that the initiation of bone resorption and formation of resorption lacunae are two independently controlled processes that require different classes of proteinases. Cysteine proteinases are required for degradation of matrix proteins in the resorption lacunae. Inhibition of cysteine proteinases produces abnormal pits but does not affect the surface area of bone resorbed. Interstitial collagenase, in contrast, is essential for the initiation of bone resorption in this system but not for degradation of mineralized matrix.
Several cysteine proteinases (cathepsins) have been investigated for their possible involvement in bone resorption (7, 36, 37). The recently discovered cathepsin K appears to be the most abundant cathepsin produced by osteoclasts (5, 38, 39), and human mutations in cathepsin K produce severe abnormalities in bone resorption (6). In this study we have provided direct experimental evidence that cysteine proteinases are required to degrade bone matrix proteins but are not required for osteoclast activation.
Several prior studies have indicated that interstitial collagenase is required for bone resorption (3, 8, 17, 18). The most widely held view has been that collagenase removes unmineralized osteoid, allowing osteoclasts to adhere to mineralized bone which triggers bone-resorptive activity (8, 17, 18). The present study provides evidence against this model, since the dentine slices have no unmineralized matrix layer, the presence or absence of interstitial collagenase activity had no effect on the number of adherent osteoclasts, and the addition of predigested gelatin to the bone slices stimulated resorption even in the presence of metalloproteinase inhibitor.
Our results indicate an alternative mechanism: that interstitial
collagenase generates collagen degradation fragments that activate
osteoclasts to resorb bone. What precisely does collagenase cleavage do
to trigger bone resorption? Precoating dentine slices with
heat-denatured but uncleaved gelatin restored normal bone resorption in
the presence of collagenase inhibitors, suggesting that crucial key
event is loss of the helical collagen structure. Collagen has binding
sites for 2
1 and
V
3 integrins, both of which are found on
the surface of osteoclasts. A recent study found that osteoclasts
adhere to undenatured collagen through
2
1
and to denatured collagen through
V
3;
adherence to the two different substrates coated on glass coverslips
produced distinct physiologic changes in osteoclasts (40). Hence,
collagenase cleavage of collagen, which results in a loss of helical
collagen structure at 37 °C (41), could expose
V
3 binding sites, an event that may be
involved in osteoclast activation.
The predominant human collagenase in most human tissues, collagenase-1 (MMP-1), cleaves helical collagen but has little telopeptidase or gelatinolytic activity (21, 42). In transgenic mice mutated to disrupt the cleavage site in helical collagen, however, only modest abnormalities of bone remodeling were observed (43), suggesting that proteinases with substrate specificities different from human MMP-1 may be involved in bone remodeling. The substrate specificity of interstitial collagenase (MMP-13), the only collagenase in rodents, differs significantly from human MMP-1; it possesses telopeptidase and gelatinolytic activity in addition to cleaving helical collagen (43). An analogous human collagenase (collagenase-3; MMP-13) recently identified in human chondrocytes (44, 45), appears to be the human homolog of rodent interstitial collagenase. Our studies suggest the possibility that the telopeptidase and gelatinolytic activities of MMP-13 may have an essential role in activating human bone resorption. As collagenase was detectable only in osteoblasts and other non-osteoclastic cells, the enzyme may function as a "coupling factor" allowing osteoblasts to exert control over osteoclast resorptive activity.
We thank Royana Lin for assistance in some experiments and Drs. Louis Avioli and Dwight Towler for comments on the manuscript.