Distribution of Small Integrin-Binding LIgand, N-linked Glycoproteins (SIBLING) in the condylar cartilage of rat mandible

Abstract

The Small Integrin-Binding LIgand, N-linked Glycoprotein (SIBLING) family is one category of non-collagenous proteins closely related to osteogenesis. In this study, the authors systematically evaluated the presence and distribution of four SIBLING family members, dentin sialophosphoprotein (DSPP), dentin matrix protein 1 (DMP1), bone sialoprotein (BSP) and osteopontin (OPN), in rat mandibular condylar cartilage using protein chemistry and immunohistochemistry. For protein chemistry, SIBLING proteins in the dissected condylar cartilage were extracted with 4 M guanidium–HCl, separated by ion-exchange chromatography, and analyzed by Western immunoblotting. Immunohistochemistry was employed to assess the distribution of these four SIBLING proteins in the condylar cartilage of 2-, 5- and 8-week-old rats. Results from both approaches showed that all four members are expressed in the condylar cartilage. DSPP, unlike that observed in dentin and bone, exists as a full-length form (uncleaved) in the condylar cartilage. The NH 2 -terminal fragment of DMP1 is mainly detected in the matrix of the cartilage while the COOH-terminal fragment is primarily localized in the nuclei of cells in the chondroblastic and hypertrophic layers. The data obtained in this investigation provide clues about the potential roles of these SIBLING proteins in chondrogenesis.

Mandibular condylar cartilage is categorized as an articular cartilage, but is distinguished from the articular cartilages of the long bones in many aspects, such as embryonic origin, ontogenetic development, post-natal growth mode and histological structure . As an important growth site for the mandible, the condylar cartilage is divided into five layers: articular, prechondroblastic, chondroblastic, hypertrophic and cartilage–bone interface . In the condylar cartilage of rat, cell proliferation and extracellular matrix (ECM) production contribute to the growth of articular cartilage and subarticular layers. In addition to collagen and water, the ECM of the condylar cartilage contains a number of non-collagenous proteins (NCPs) and proteoglycans. The Small Integrin-Binding LIgand, N-linked Glycoprotein (SIBLING) family is one category of NCPs, which includes dentin sialophosphoprotein (DSPP), dentin matrix protein 1 (DMP1), bone sialoprotein (BSP), osteopontin (OPN), and matrix extracellular phosphoglycoprotein (MEPE). Principally found in mineralized tissues, SIBLING family members are thought to play important roles in the formation of bone and dentin .

DSPP, originally thought to be tooth-specific, is now found in the bone, cementum and some non-mineralized tissues at a remarkably lower level than in the dentin . In the ECM of dentin, DSPP is present as proteolytically processed fragments, dentin sialoprotein (DSP) and dentin phosphoprotein (DPP), which originate from the NH 2 -terminal and COOH-terminal regions of the DSPP amino acid sequence, respectively . While DSP and DPP are abundant in the ECM of dentin , the intact, full-length form, representing the whole sequence of DSPP, has never been identified. Gene ablation experiments in mice have demonstrated that DSPP and/or its processed fragments (DSP and DPP) are critical for the mineralization of dentin . The exact mechanisms by which DSPP functions in biomineralization are unknown.

DMP1 is an acidic phosphoprotein predominantly expressed in dentin, bone and cementum . A lower level of expression for this protein has also been found in non-mineralized tissues such as the brain, kidney, pancreas, and salivary glands . Like DSPP, DMP1 in the ECM of bone and dentin mainly occurs as proteolytically processed 37 kDa fragments and 57 kDa fragments, which originate from the NH 2 -terminal and COOH-terminal regions of the DMP1 amino acid sequence, respectively . Recently, the full-length form of DMP1 has been identified in the ECM of rat dentin and bone, the concentration of which is considerably lower than its processed fragments in these two tissues . The importance of DMP1 for dentin and bone mineralization has been demonstrated by gene ablation experiments in mice and in human genetic mutation studies .

Bone sialoprotein is primarily found in bone, mineralizing cartilage, cementum, and reactionary dentin . The biological functions of BSP in mineralized tissues are largely unknown. Some data suggest that BSP acts as a nucleator for the formation of initial apatite crystals, and then, as this mineral grows on the collagen matrix, it acts as an inhibitor in directing the growth of the crystals .

OPN is present in relatively large quantities in non-mineralized tissues as well as mineralized tissues. In mineralized tissues, OPN is expressed in bone, cementum, predentin, and tertiary dentin . In vitro and in vivo studies show that OPN is an effective inhibitor of apatite formation and growth .

There is a large body of information about the biochemical properties and tissue expression of SIBLING family members in bone and dentin but little is known about these molecules, especially DSPP and DMP1, in the mandibular condylar cartilage. The main objectives of this investigation are to evaluate the presence or absence of the four SIBLING members and their relative expression level in the condylar cartilage of the rat mandible, and the difference in the expression pattern of these SIBLING family members and/or their processed fragments in association with the anatomical structure of the cartilage during post-natal growth. In this study, using protein chemistry and immunohistochemistry approaches the authors detected DSPP, DMP1, BSP and OPN in the rat condylar cartilage, which show remarkable variations between different layers of cartilage and at different ages. These findings provide novel information and clues about the potential roles of these molecules in the chondrogenesis of condylar cartilage and osteogenesis of the mandibular ramus.

Materials and methods

Tissue acquisition/extraction of NCPs

Sprague–Dawley rats (Harlan, Indianapolis, IN, USA) aged 2, 5, 8 and 12 weeks were used in this study. Mandibular condylar cartilage tissues from the 2-, 5- and 8-week-old rats were used for immunohistochemistry (IHC) staining while those from 12-week-old rats were used for protein chemistry analysis. The animal protocol was approved by the Animal Welfare Committee of Baylor College of Dentistry of the Texas A & M University System Health Science Center.

Extraction and separation of NCPs of the mandibular condylar cartilage

Twenty 12-week-old rats (40 mandibular condyles) were used for the extraction of NCPs. The condylar cartilage was carefully separated at the cartilage–bone interface under a dissecting microscope. The procedure for protein extraction and separation from the cartilage was similar to that routinely employed in the laboratory for extracting proteins from bone and dentin . Briefly, the condylar cartilage was placed in 4 M guanidium–HCl (Gdm–HCl; Acros Organics, Fairlawn, NJ, USA) solution (pH 7.2) containing proteinase inhibitors for 48 h. This procedure extracts NCPs (including the SIBLING family members) from the unmineralized phase (i.e. the condylar cartilage). NCPs in the mineralized phase cannot be extracted by Gdm–HCl without demineralization reagents. This protocol ensures that if there is a minor amount of contaminating mineralized tissue (mineralized cartilage or bone), the NCPs from the mineralized phase will not contaminate the samples from the non-mineralized cartilage. The Gdm–HCl extracts were subjected to Q-Sepharose (Amersham Biosciences, Uppsala, Sweden) ion-exchange chromatography with a gradient ranging from 0.1 M to 0.8 M NaCl in a 6 M urea solution of pH 7.2. Acidic proteins from this extraction were eluted into sequential fractions, each in 1.0 ml of 6 M urea solution. Each separated chromatographic fraction in 6 M urea solution was analyzed by sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE). Stains-All staining and Western immunoblotting were carried out to evaluate the presence of DSPP, DMP1, BSP, OPN and their processed fragments.

SDS-PAGE and Western immunoblotting

For SDS-PAGE, 5–15% gradient gels were used in all the experiments. 60 μl of sample from each chromatographic fraction was loaded onto the gels. Stains-All staining was used for detecting the ECM proteins eluted from ion-exchange chromatography. For Western immunoblotting detection of DSPP/DSP, an anti-DSP polyclonal antibody ( Table 1 ) was used at a dilution of 1:3000 in blocking buffer. For detection of DMP1, two types of anti-DMP1 antibodies were used. One was a monoclonal antibody generated using the NH 2 -terminal fragment of rat bone DMP1 as the antigen (designated as anti-DMP1-N-9B6.3, immunoreactive to the NH 2 -terminal region of DMP1 ) and was used at a dilution of 1:1000. The other was a polyclonal antibody referred to as anti-DMP1-C-857, which recognizes the COOH-terminal region of DMP1 and was used at a dilution of 1:2000. For detection of BSP, a monoclonal anti-BSP antibody known as anti-BSP-10D9.2 was used at a dilution of 1:2000. For detection of OPN, an anti-OPN polyclonal antibody was used at a dilution of 1:2000. Blots were washed three times in PBS containing 0.3% tween-20, and followed by incubation in secondary antibody with a 1:5000 dilution of alkaline phosphate-conjugated anti-mouse IgG or anti-rabbit IgG (Sigma–Aldrich, Louis, MO, USA). The blots were incubated in the chemiluminescent substrate CDP-star (Ambion, Austin, TX, USA) for 5 min and exposed to X-ray films.

Table 1
Antibodies used in this study.
Antibody Antibody type Immunizing antigen Immunoreactivity in Western blotting Immunoreactivity in immunohistochemistry
Anti-DSP-2C12.3 a Monoclonal Purified rat dentin DSP No Yes
Anti-DSP b Polyclonal Purified rat dentin DSP Yes Yes
Anti-DMP1-N-9B6.3 c Monoclonal 37 kDa (N-terminal) Yes Very weak
Anti-DMP1-N-859 d Polyclonal Oligopeptide (residues 101–121) Yes Yes
Anti-DMP1-C-8G10.3 e Monoclonal 57 kDa (C-terminal) No Yes
Anti-DMP1-C-857 f Polyclonal Oligopeptide (residues 471–485) Yes Yes
Anti-BSP-10D9.2 g Monoclonal Purified rat bone BSP Yes Yes
Anti-OPN h Polyclonal Recombinant rat OPN Yes Yes

a This monoclonal antibody was used to detect DSP by immunohistochemistry analysis.

b This polyclonal antibody was used to detect DSP by Western immunoblotting.

c This monoclonal antibody was used to detect the NH 2 -terminal fragment of DMP1 by Western immunoblotting analysis.

d This polyclonal antibody was used to detect the NH 2 -terminal fragment of DMP1 by immunohistochemistry and immunofluorescence analysis.

e This monoclonal antibody was used to detect the COOH-terminal fragment of DMP1 by immunohistochemistry and immunofluorescence analysis.

f This polyclonal antibody was used to detect the COOH-terminal fragment of DMP1 by Western immunoblotting analysis.

g This monoclonal antibody was used to detect BSP by immunohistochemistry analysis and Western immunoblotting.

h This polyclonal antibody was used to detect OPN by immunohistochemistry analysis and Western immunoblotting.

Immunohistochemistry (IHC)

IHC was performed to analyze the difference in the expression and distribution pattern of these SIBLING proteins in the mandibular condylar cartilage from 2-, 5- and 8-week-old rats. Under anesthesia, Sprague–Dawley rats (Harlan, Indianapolis, IN, USA) at the above ages were perfused from the ascending aorta with 4% paraformaldehyde in 0.1 M phosphate buffer. The mandibles were dissected and further fixed in the same fixative for 48 h, followed by decalcification in 8% EDTA (pH 7.4) at 4 °C for approximately 4 weeks. Tissues were processed for paraffin embedding, and serial 5 μm sections were prepared. For immunohistochemical detection of DSPP/DSP: the anti-DSP monoclonal antibody designated as anti-DSP-2C12.3 ( Table 1 ) was used at a dilution of 1:200. For DMP1, two types of antibodies were used at a dilution of 1:300: a monoclonal antibody referred to as anti-DMP1-C-8G10.3 , which specifically recognizes the COOH-terminal fragment of DMP1 in IHC; the other was a polyclonal antibody known as anti-DMP1-N-859 , which recognizes the NH 2 -terminal fragment of DMP1. For BSP and OPN, antibodies were identical to those used in Western immunoblotting, and the dilution was 1:200. All IHC experiments were carried out using ABC kit and DAB kit (Vector Laboratories Inc., Burlingame, CA, USA), following the manufacturer’s instructions.

Immunofluorescence analysis of DMP1 fragments

A double immunofluorescent staining approach was used to detect the location differences of DMP1 fragments in the condylar cartilage of rat mandible. The sections were first incubated with a mixture of the two primary antibodies, anti-DMP1-N-859 and anti-DMP1-C-8G10.3 (each diluted at 1:400), which recognize the NH 2 -terminal and COOH-terminal regions of DMP1, respectively. The sections were incubated with goat anti-rabbit F (ab’) 2 fragment conjugated with Alexa 488 (green) and goat anti-mouse F(ab’) 2 fragment conjugated with Alexa 546 (red, both from Invitrogen, Camarillo, CA, USA) at a dilution of 1:600. Nuclei were counterstained with TO-PRO-3 (Invitrogen, CA, USA) at a dilution of 1:500 for 5 min to stain the nuclei (for blue colour). After mounting with Slowfade, the images were captured and analyzed with a Leica TCS-SP2 confocal microscope (Heidelberg, Germany).

Table 1 is a summary of the antibodies used in this study. Detailed information for all of these antibodies can be found in the authors’ previous publications .

Results

DSPP, DMP1, BSP and OPN in the Gdm–HCl extracts of the condylar cartilage

Q-Sepharose ion-exchange chromatography separated Gdm–HCl extracts of the cartilage into 120 fractions ( Fig. 1 ). Each of the chromatographic fractions that might potentially contain any of the four SIBLING family members was assayed by Stains-All staining and Western immunoblotting. In this report, the Stains-All staining of fractions 15 through 93 is presented ( Fig. 2 ) to illustrate the results. To show the identity of DSPP/DSP, Western immunoblotting of fractions 27 through 39 is shown while for that of the other three SIBLING family members, Western immunoblotting of one representative fraction is shown ( Fig. 3 ).

Fig. 1
Separation of NCPs extracted from the rat mandibular condylar cartilage. Q-Sepharose ion-exchange chromatography separated NCPs extracted from rat mandibular condylar cartilage into 120 fractions. Each fraction contained 1 ml of 6 M urea solution.

Fig. 2
Stains-All staining for chromatographic fractions 15–93 of the Gdm–HCl extract from the rat mandibular condylar cartilage. Digits at the top of the figure represent fraction numbers. The blue protein bands in fractions 48–54 migrating between the 53 kDa and 78 kDa molecular weight markers represent OPN. The blue protein bands around 80 kDa (between the 78 kDa and 114 kDa markers) in fractions 54–81 represent BSP. The identification of these Stains-All positive protein bands as OPN and BSP was confirmed by Western immunoblotting (see Fig. 3 ).

Fig. 3
Western immunoblotting for DSPP and its fragments, DMP1 and its fragments, BSP and OPN. (A) Western immunoblotting using anti-DSP polyclonal antibody for fractions 27–39 of Q-Sepharaose chromatography of NCPs extracted from rat condylar cartilage. Positive control (Cont): 0.3 μg of DSP isolated from rat incisor dentin; 27–39: 60 μl of sample from fractions 27–39 were treated with 2.5% of β-mercaptoethanol before loading. Long arrow indicates the migrating position of full-length DSPP; arrowhead indicates the migrating position of DSP. (B) Western immunoblotting using anti-DMP1-N-9B6.3 monoclonal antibody. Cont: 1 μg of the NH 2 -terminal (37 kDa) fragment of DMP1 and the full-length form of DMP1 isolated from rat long bone. 51: 60 μl of sample from fraction 51 of Q-Sepharaose chromatography of NCPs extracted from rat condylar cartilage. Both the 37 kDa fragment (arrowhead) and full-length form of DMP1 (long arrow) are detected in the extract from the rat condylar cartilage. In comparison with the DMP1 molecular species in the extract from rat long bone (Cont in B), the full-length form of DMP1 is more abundant in the extract from the cartilage. (C) Western immunoblotting using anti-DMP1-C-857 polyclonal antibody. Cont: 1 μg of the COOH-terminal (57 kDa) fragment and the full-length form of DMP1 isolated from rat long bone. 51: 60 μl of sample from fraction 51 of Q-Sepharaose chromatography of NCPs extracted from rat condylar cartilage. While the full-length form of DMP1 (long arrow) was visualized, the 57 kDa fragment (arrowhead) was hardly detectable in the extract from the rat condylar cartilage. (D) Western immunoblotting using anti-BSP-10D9.3 monoclonal antibody. Cont: 1 μg of BSP isolated from rat long bone. 69: fraction 69 of Q-Sepharaose chromatography of NCPs extracted from rat condylar cartilage. Arrow indicates the migrating position of BSP. (E) Western immunoblotting using the anti-OPN polyclonal antibody. Cont: 1 μg of OPN isolated from rat long bone. 51: fraction 51 of Q-Sepharaose chromatography of NCPs extracted from rat condylar cartilage. Arrow indicates the migrating position of OPN.

Stains-All staining failed to demonstrate any protein bands corresponding to the migration rates of DSPP, DSP or DPP on SDS-PAGE ( Fig. 2 ), whereas on Western immunoblotting, a clear band in fractions 27–37 corresponding to the migration rate of the full-length form of DSPP (180–190 kDa) was recognized by the anti-DSP antibody ( Fig. 3 A). This observation indicated that the amount of DSPP in the sample was not sufficient for disclosure by Stains-All staining, but could be clearly detected by Western immunoblotting. The migration rate of the protein bands in fractions 27–39 that were immunoreactive to the anti-DSP antibody were identical to the full-length form of mouse recombinant DSPP made in HEK-293 cells, which migrates between 180 kDa and 190 kDa on 5–15% gradient gel (Sun and Qin, unpublished data). Before loading onto SDS-PAGE, the sample was treated with 2.5% β-mercaptoethanol to eliminate the disulphide-bond linked dimeric form of DSP; previous studies have shown that dentin ECM contain a dimeric form of DSP that migrates over 200 kDa on SDS-PAGE . Taken together, the authors concluded that this 180–190 kDa protein band in fractions 27–39 ( Fig. 3 A) represented the full-length form of DSPP. DSP (the NH 2 -terminal fragment of DSPP) was hardly detectable in any of the chromatographic fractions (including fractions prior to 27). This observation clearly indicated that the majority of DSPP is not cleaved in the condylar cartilage of the rat mandible, which differs from the data obtained from dentin ECM, in which DSPP is hardly detectable whereas its cleaved products DSP and DPP are abundant.

Previous studies showed that during ion-exchange chromatography, the NH 2 -terminal (37 kDa) and COOH-terminal (57 kDa) fragments of DMP1 and the full-length form of DMP1 co-elute with OPN . In this investigation, Western immunoblotting using the anti-DMP1-N-9B6.3 antibody showed the presence of the full-length form and the NH 2 -terminal (37 kDa) fragment of DMP1 ( Fig. 3 B) in the fractions, in which OPN eluted. The anti-DMP1-C-857 antibody (immunoreactive to the COOH-terminal region of DMP1) could hardly detect the 57 kDa fragment but clearly demonstrated the presence of the full-length form of DMP1 ( Fig. 3 C) in these fractions; a faint 57 kDa band could be observed only when a very large volume of sample was loaded or when the X-ray film was exposed for a prolonged period of time. The full-length form of DMP1 (long arrows in Fig. 3 B and C) was detected by both the anti-DMP1-N-9B6.3 and anti-DMP1-C-857 antibodies in Western immunoblotting. In the condylar cartilage, the full-length form of DMP1 appeared more abundant than its processed fragments.

The protein band representing BSP was clearly observed in fractions 57–81 by Stains-All staining ( Fig. 2 , the blue protein band migrating between the 78 kDa and 114 kDa markers). The identification of this protein band as BSP was further confirmed by Western immunoblotting using the anti-BSP-10D9.2 antibody ( Fig. 3 D).

In the Q-Sepharose chromatography of Gdm–HCl extract from the rat condylar cartilage, OPN mainly eluted in fractions 48–54 and was clearly detected in these fractions by Stains-All staining ( Fig. 2 , the most remarkable blue protein band migrating just below the 78 kDa molecular weight marker in fractions 48–54). Western immunoblotting further confirmed the abundance of this protein in the condylar cartilage. A broad, dark protein band below the 78 kDa molecular marker was recognized by the anti-OPN antibody ( Fig. 3 E).

Immunohistochemistry (IHC)

The condylar cartilage of the mandible can be divided into five layers based on histological appearance ( Fig. 4 A1–A3 ): articular (Ar), prechondroblastic (Pr), chondroblastic (Ch), hypertrophic (Hy) and cartilage–bone interface (C–B). At 5 weeks after birth, the condylar cartilage is wider than at 2 or 8 weeks. Immunohistochemical staining showed that each of the four SIBLING family members had its own preference for distribution in specific layers, although all of them were detected in the cartilage. The distribution patterns also changed in relation to post-natal growth of the animals.

Fig. 4
H&E and IHC staining for paraffin sections of the condylar cartilage from 2-, 5- and 8-week-old rats. Column 1, 2-week-old rat; column 2, 5-week-old rat; column 3, 8-week-old rat. Ar, articular layer; Pr, prechondroblastic layer; Ch, chondroblastic layer; Hy, hypertrophic layer; C–B, cartilage–bone interface. Row A, H&E staining; row B, IHC for DSPP; row C, IHC for the NH 2 -terminal fragment of DMP1; row D, IHC for the COOH-terminal fragment of DMP1; row E, IHC for BSP; row F, IHC for OPN. Bar equals 100 μm in all microphotographs. DSPP was observed in the cells of all five layers and in the ECM of the articular layer and prechondroblastic layer at 2 weeks (B1). At 5 and 8 weeks (B2 and B3), the signal for DSPP was detected in the cells of the chondroblastic and hypertrophic layers, as well as in the ECM of the articular, prechondroblastic and chondroblastic layers. The signal for the NH 2 -terminal fragment of DMP1 was mainly observed in the ECM of the articular layer and prechondroblastic layer at 2 weeks (C1). At 5 and 8 weeks (C2 and C3), the signal for the NH 2 -terminal fragment of DMP1 was mainly observed in the cells and the ECM of the chondroblastic and hypertrophic layers. Note that the IHC staining in the 5-week-old group is weaker than in the 8-week-old group. The signal for the COOH-terminal fragment of DMP1 (D1–D3) was primarily observed in the nuclei of cells of the chondroblastic and upper part of the hypertrophic layers. BSP was observed in the cells of all five layers and in the ECM of the articular layer at 2 weeks (E1). At 5 weeks (E2), BSP signal was strong in the nuclei of cells in the prechondroblastic and chondroblastic layers and in the ECM of all five layers. At 8 weeks (E3), the signal for BSP was mainly observed in the prechondroblastic, chondroblastic and hypertrophic layers. OPN was observed in the cells of all five layers and in the ECM of the articular layer at 2 weeks (F1). At 5 and 8 weeks (F2 and F3), the signal for OPN was mainly observed in the nuclei of the chondroblastic layer and in the ECM of the prechondroblastic and chondroblastic layers.

DSPP was most pronounced within the cells in the articular layer and prechondroblastic layer at 2 weeks after birth, although the signal for DSPP could be observed across the whole area of the cartilage ( Fig. 4 B1). At 5 and 8 weeks ( Fig. 4 B2 and B3), DSPP was more prominent in the chondroblastic layer and the upper hypertrophic layer than in the superficial layer. DSPP was found in the ECM as well as within the cells.

The signal for the NH 2 -terminal fragment of DMP1 was very strong in the ECM of the articular and prechondroblastic layers but weaker in the chondroblastic and hypertrophic layers of the cartilage, 2 weeks after birth ( Fig. 4 C1). At 5 weeks, the signal for the NH 2 -terminal fragment of DMP1 decreased across all layers of cartilage ( Fig. 4 C2), whereas at 8 weeks, the signal for the NH 2 -terminal fragment of DMP1 increased in the ECM of the prechondroblastic and chondroblastic layers ( Fig. 4 C3).

While the signal for the COOH-terminal fragment of DMP1 was weak across all layers of the condylar cartilage at 2 and 8 weeks after birth ( Fig. 4 D1 and D3), at 5 weeks a relatively strong immunoreactivity for this fragment was observed within the nuclei of cells in the chondroblastic layer and upper part of the hypertrophic layer adjacent to the chondroblasts ( Fig. 4 D2).

BSP was observed in significant amounts in all of the five layers of the condylar cartilage from all of the three age groups ( Fig. 4 E1–E3). At 5 weeks, the signal for BSP was very strong in the ECM of the prechondroblastic and chondroblastic layers and within the cells of these two layers ( Fig. 4 E2).

At 2 weeks, OPN was prominent in the articular layer ( Fig. 4 F1), while at 5 weeks this protein was mainly detected in the cells of the chondroblastic layer ( Fig. 4 F2). The signal for OPN in the chondroblastic layer of the condylar cartilage from the 8-week-old rat ( Fig. 4 F3) appeared stronger than the level at 5 weeks. The IHC results are summarized in Table 2 .

Feb 8, 2018 | Posted by in Oral and Maxillofacial Surgery | Comments Off on Distribution of Small Integrin-Binding LIgand, N-linked Glycoproteins (SIBLING) in the condylar cartilage of rat mandible

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