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© The Rockefeller University Press,
0021-9525/2001//87 $5.00
The Journal of Cell Biology, Volume 153, Number 1,
, 2001 87-100
Original Article |
Skeletal Malformations Caused by Overexpression of Cbfa1 or Its Dominant Negative Form in Chondrocytes
komorit{at}imed3.med.osaka-u.ac.jp
During skeletogenesis, cartilage develops to either permanent cartilage that persists through life or transient cartilage that is eventually replaced by bone. However, the mechanism by which cartilage phenotype is specified remains unclarified. Core binding factor
1 (Cbfa1) is an essential transcription factor for osteoblast differentiation and bone formation and has the ability to stimulate chondrocyte maturation in vitro. To understand the roles of Cbfa1 in chondrocytes during skeletal development, we generated transgenic mice that overexpress Cbfa1 or a dominant negative (DN)-Cbfa1 in chondrocytes under the control of a type II collagen promoter/enhancer. Both types of transgenic mice displayed dwarfism and skeletal malformations, which, however, resulted from opposite cellular phenotypes. Cbfa1 overexpression caused acceleration of endochondral ossification due to precocious chondrocyte maturation, whereas overexpression of DN-Cbfa1 suppressed maturation and delayed endochondral ossification. In addition, Cbfa1 transgenic mice failed to form most of their joints and permanent cartilage entered the endochondral pathway, whereas most chondrocytes in DN-Cbfa1 transgenic mice retained a marker for permanent cartilage. These data show that temporally and spatially regulated expression of Cbfa1 in chondrocytes is required for skeletogenesis, including formation of joints, permanent cartilages, and endochondral bones.
Key Words: chondrocyte • Cbfa1 • transgenic mice • endochondral ossification • permanent cartilage
© 2001 The Rockefeller University Press
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Introduction |
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Core binding factor 1 (Cbfa1)/Runx2 (runt-related gene 2) is an essential transcription factor in osteoblast differentiation and bone formation (Ducy et al. 1997; Komori et al. 1997; Otto et al. 1997). Cbfa1-deficient mice display a complete lack of both intramembranous and endochondral ossification and show an absence of osteoblast differentiation, as well as retardation of chondrocyte differentiation (Komori et al. 1997; Otto et al. 1997; Inada et al. 1999; Kim et al. 1999). Further, Cbfa1 has the ability to stimulate chondrocyte maturation in vitro (Enomoto et al. 2000). Thus, a main function of Cbfa1 in chondrocytes in vivo appears to be promotion of their maturation and endochondral ossification. However, it may be that chondrocyte differentiation leading to endochondral ossification is largely controlled by the surrounding cells, osteoblastic and hematopoietic cells, and that a lack of Cbfa1 in chondrocytes may not be a major reason for suppression of chondrocyte maturation. Thus, the mechanism of inhibition of endochondral ossification seen in Cbfa1-deficient mice remains to be solved.
To examine the roles of Cbfa1 in endochondral ossification and cartilage phenotype specification, we generated transgenic mice, which overexpress Cbfa1 or a dominant negative (DN)-Cbfa1 form in chondrocytes under the control of promoter/enhancer elements of the 1 type II collagen gene (Col2a1). Cbfa1 and DN-Cbfa1 transgenic mice showed, respectively, accelerated and decelerated chondrocyte maturation and endochondral ossification. Further, permanent cartilage lost its permanent phenotype and entered into the endochondral process in Cbfa1 transgenic mice, whereas most of the chondrocytes in DN-Cbfa1 transgenic mice retained the phenotype of permanent cartilage. These data demonstrate that Cbfa1 plays an important role not only in chondrocyte maturation in the process of endochondral ossification, but also in the specification of cartilage phenotype.
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Materials and Methods |
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DNA Transfections and Luciferase Assays
Type I Cbfa1, type II Cbfa1, and DN-Cbfa1 (673-bp BamHI-HindIII fragment) were subcloned into the pSG5 vector (Stratagene) as described (Harada et al. 1999) and designated pSG5-type I Cbfa1, pSG5-type II Cbfa1, and pSG5–DN-Cbfa1, respectively. Insertless pSG5 vector (pSG5) was used as a control expression vector. A pGL3 promoter vector (Promega), containing six repeats of the consensus Cbfa1 binding sites, was used as an experimental reporter vector (p6XOSE2-Luc) (Harada et al. 1999). A pRL-SV40 vector (Promega) was used as a control reporter vector. Subconfluent cultures of chick sterna chondrocytes in a 6-well plate were transfected with 0.5 µg of p6XOSE2-Luc, 0.2 µg of pRL-SV40, and 3.3 µg of a mixture of pSG5 expression vectors with LipofectAMINE 2000 reagent (GIBCO BRL). After 48 h, cells were harvested and firefly luciferase activities generated by experimental reporter, and Renilla luciferase activity generated by control reporter, were simultaneously measured by Dual-Luciferase reporter assay system (Promega). The value of reporter gene activity was calculated by dividing firefly luciferase activity by Renilla luciferase activity and the result was expressed as relative luciferase activity. Transfection and reporter gene assay were carried out according to the manufacturer's protocol.
Skeletal, Histological, and Immunohistochemical Examinations
For staining and visualization of the whole skeleton, cleared skeletons of E15.5–18.5 embryos were stained with Alizarin red–S and Alcian blue as described (Komori et al. 1997). For light microscopy, tissues from E12.5–18.5 embryos were fixed in 4% paraformaldehyde/0.1 M phosphate buffer. Sections (7 µm in thickness) were stained with hematoxylin and eosin (H-E). Selected samples were stained using von Kossa's method to identify mineralized tissues (Komori et al. 1997). For immunohistochemical analysis, the sections were pretreated with 0.2% pepsin in 0.02 N HCl for 15 min at 37°C and then incubated with rabbit anti–mouse tenascin antibody (Kalembey et al. 1997) for 16 h at 4°C. Localization of the first antibody was visualized by incubation with biotinylated anti–rabbit IgG (Vector Laboratories) for 30 min at room temperature and then with Cy3-conjugated Streptavidin (Jackson ImmunoResearch Laboratories) for 30 min at room temperature.
Detection of β-Galactosidase Activity
For the detection of β-galactosidase activity, embryos were fixed with 4% paraformaldehyde in PBS (pH 7.4) at 4°C for 20 min. The samples were then rinsed in PBS, subsequently transferred into X-gal reaction mixture (1 mg/ml 4-chloro-5-bromo-3-indolyl-β, 4 mM K4Fe[CN]63H2O, 4 mM K3Fe[CN]6, 2 mM MgCl2 in PBS), and incubated at 30°C overnight. Stained embryos were embedded in paraffin and used to generate 7-µm sections, which were counterstained with eosin.
In Situ Hybridization
Digoxigenin 11 UTP-labeled single-stranded RNA probes were prepared using a DIG RNA labeling kit (Roche Biochemica) according to the manufacturer's instructions. A 0.4-kb fragment of mouse 1(II) collagen cDNA (Komori et al. 1997), a 0.65-kb fragment of mouse 1(X) collagen cDNA (Inada et al. 1999), a 0.8-kb fragment of mouse parathyroid hormone/parathyroid hormone–related peptide (PTH/PTHrP) receptor cDNA (Inada et al. 1999), a 0.6-kb fragment of mouse Indian hedgehog (Ihh) cDNA (Inada et al. 1999), and a 0.27-kb fragment of mouse growth and differentiation factor (GDF)-5 cDNA were used to generate antisense and sense probes. Hybridization was carried out as described (Inada et al. 1999).
Cell Cultures and Virus Infection
Chick sterna chondrocytes were isolated from 17-d-old embryo (line M) sternum, infected with the RCAS retroviral vector encoding type I Cbfa1, or the runt domain with NH2-terminal domain of type I Cbfa1, and cultured in high-glucose DME containing 10% FBS and 10 µg/ml of ascorbic acid as described previously (Enomoto-Iwamoto et al. 1998; Enomoto et al. 2000). On day 5, the cultures were replated in 24-well plates or 60-mm dishes at the density of 3 x 105 per well and 106 per dish, respectively. After 5 d the cultures in 60-mm dishes were subjected to immunoblot and Northern blot analyses (Inada et al. 1999). The cultures in 24-well plates were maintained for 8 d, then treated with 3 mM β-glycerophosphate for the additional 2 d and fixed for histochemical examination (Enomoto et al. 2000). The first antibody used was a polyclonal rabbit antibody against the NH2-terminal domain of type I Cbfa1, provided by Y. Ito (Kyoto University, Kyoto, Japan). Chick type II collagen, type X collagen, and tenascin cDNAs used for probes were described previously (Pacifici et al. 1993).
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A (hereafter termed type I Cbfa1; Ogawa et al. 1993); the other, translated from exon 1, was called til-1 isoform (hereafter termed type II Cbfa1; Stewart et al. 1997). Mice overexpressing type I or II Cbfa1 died at birth from respiratory failure. At E18.5, they displayed severe dwarfism, with shortened limbs, domed skull, and a protruding tongue with a shortened snout and mandible (Fig. 1 C). Most skeletal elements, including the chondrocranium, ribs, and vertebrae, showed massive mineralization with severely reduced cartilaginous portions, and the thoracic cage was narrow and bell-shaped (Fig. 2B, Fig. C, Fig. F, Fig. G, Fig. J, and Fig. K). As to be expected, age-matched wild-type mice displayed cartilaginous tissues in the joints, ventral portion of ribs, and vertebral bodies (Fig. 2A, Fig. E, Fig. I, and Fig. M). In addition, most skeletal elements in the transgenic mice were fused, except manus and pedis (Fig. 2B and Fig. C). Shoulder, elbow, hip, and knee joints were absent, and the vertebral bodies and arches were fused (Fig. 2J, Fig. K, Fig. N, and Fig. O). The overall phenotypes of type I and II Cbfa1 transgenic mice were generally similar, although type II Cbfa1 transgenic mice seemed to develop these severe abnormalities slightly earlier than type I Cbaf1 transgenic mice (Fig. 3).
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Overexpression of Cbfa1 Induced Precocious or Abnormal Endochondral Ossification
Developmental changes in cartilaginous skeletal elements were examined histologically. In E18.5 wild-type mice, nasal septum cartilage consisted of small homogenous chondrocytes (Fig. 5 A), which is typical of permanent cartilage, whereas that of Cbfa1 transgenic mice was mostly composed of hypertrophic chondrocytes and about half of it had already been replaced by bone marrow and osteoid tissues (Fig. 5 B). In wild-type mice at E18.5, the vertebral cartilage primordia just started to develop and consisted of homogenous small chondrocytes sandwiched between smaller mesenchymal cells destined to become intervertebral discs (Fig. 5 C). In Cbfa1 transgenic mice, vertebral cartilage had largely been replaced by bone, and chondrocyte maturation and bone formation were also observed in the presumed intervertebral regions (Fig. 5 D). In wild-type mice at E18.5, thyroid, cricoid, and tracheal cartilages, all of which have the permanent phenotype, consisted of small homogeneous chondrocytes (Fig. 5E and Fig. G), whereas those of Cbfa1 transgenic mice consisted of mixed populations of hypertrophic and small chondrocytes and some regions that were replaced by bone (Fig. 5F and Fig. H). Further, tracheal rings were fused in Cbfa1 transgenic mice (Fig. 5 H). These data indicate that cartilage tissues that normally develop to permanent cartilage proceeded to endochondral process in Cbfa1 transgenic mice. In the developing mandible, membranous ossification proceeds at some distance from Meckel's cartilage, the distal portion of Meckel's cartilage is replaced with fibrous tissues, and the caudal part gives rise to ossicles, such as malleus and incus, through endochondral ossification (Chung et al. 1995). However, the distal portion of Meckel's cartilage in Cbfa1 transgenic mice displayed endochondral ossification, whereas Meckel's cartilage in wild-type mice remained cartilaginous (Fig. 5, I–L). All of these findings show that chondrocyte maturation had been greatly enhanced in Cbfa1 transgenic mice, leading to abnormal behavior and development of most, if not all, cartilaginous structures.
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Discussion |
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Our data clearly demonstrate that Cbfa1 plays a crucial role in chondrocyte maturation in the process of endochondral ossification and suggest that the retardation of chondrocyte maturation in Cbfa1-deficient mice was mainly caused by a lack of Cbfa1 in chondrocytes, not a lack of osteoblast differentiation or invasion of hematopoietic cells. However, the retardation of chondrocyte maturation observed in DN-Cbfa1 transgenic mice was severer than that seen in Cbfa1-deficient mice, although bone collars in diaphyses were generated and blood vessels invaded the bone collars in DN-Cbfa1 transgenic mice. In Cbfa1-deficient mice, the entire skeleton consisted of cartilage, most of which was composed of resting or proliferating chondrocytes, which lack the expression of PTH/PTHrPR, Ihh, and type X collagen (Inada et al. 1999; Kim et al. 1999). However, chondrocyte maturation was observed in the restricted skeleton, including tibia, fibula, radius, and ulna. Calcification occurred in these areas, and PTH/PTHrPR, Ihh, and type X collagen expression was observed in their prehypertrophic and hypertrophic chondrocytes (Inada et al. 1999; Kim et al. 1999). However, in DN-Cbfa1 transgenic mice hypertrophic chondrocytes were rare throughout the skeleton. Even in the tibia, fibula, radius, and ulna, only small numbers of cells expressed PTH/PTHrPR, Ihh, or type X collagen. As DN-Cbfa1 is expected to inhibit the expression of all runt family genes including Cbfa2/Runx1 and Cbfa3/Runx3 (Sakakura et al. 1994), runt family genes other than Cbfa1 might also be involved in chondrocyte maturation.
Ihh was considered to regulate chondrocyte differentiation via PTHrP and its receptor (Vortkamp et al. 1996; Zau et al. 1997). Consequently, Ihh suppresses the differentiation of prehypertrophic chondrocytes into hypertrophic chondrocytes. As chondrocyte maturation was arrested before the prehypertrophic stage in DN-Cbfa1 transgenic mice, the maturational disturbance cannot be explained by Ihh signaling. In DN-Cbfa1 transgenic mice, delayed bone collar formation is probably due to low Ihh expression in chondrocytes (Fig. 6G and Fig. J, and Fig. 7 E), whose level is less than the detection level of in situ hybridization, because Ihh-deficient mice displayed a complete lack of bone collar formation (St.-Jacques et al. 1999). Our data also indicate that osteoblast differentiation in the perichondrial region has no significant supportive effect on chondrocyte maturation at least in the absence of runt family factors in chondrocytes. Further evidence is provided by the finding that chondrocytes became hypertrophic in the absence of osteoblast differentiation in the perichondrial region of Ihh-deficient mice (St.-Jacques et al. 1999). However, vascular invasion seemed to support chondrocyte maturation, because a few type X collagen-positive cells appeared close to hematopoietic cells that had invaded to the inside of the bone collar in DN-Cbfa1 transgenic mice (Fig. 7 H).
Cbfa1 isoforms with different NH2 termini have been shown to have different transcriptional activities in genes of bone matrix proteins, including type I collagen and osteocalcin, in vitro (Tuji et al. 1998; Harada et al. 1999), although the functional difference remains to be clarified in vivo. We could not find functional differences between Cbfa1 isoforms in chondrocyte maturation, and both isoforms strongly stimulated chondrocyte maturation. However, type II Cbfa1 seemed to exert stronger activity in stimulating chondrocyte maturation than type I Cbfa1 (Fig. 3). This was also observed during in vitro experiments using chick primary chondrocytes (Enomoto et al. 2000). Differences in the function of the two Cbfa1 isoforms in chondrocytes need to be further investigated, especially in hypertrophic chondrocytes in which Cbfa1 and matrix protein genes related to calcification are highly expressed. Cbfa1 induced the differentiation of two lineage cells, osteoblasts and chondrocytes (Komori 2000). As the two Cbfa1 isoforms are expressed in chondrocytes as well as osteoblasts, isoform-dependent induction of each lineage differentiation is not valid. It has been shown that Ets1 works cooperatively with Cbfa1 in transactivation of the osteopontin gene (Sato et al. 1998). Although transcription factors that specifically interact with Cbfa1 in chondrocytes have not been identified, it is suggested that additional transcription factors required for cooperative work with Cbfa1 are different in chondrocyte and osteoblast differentiation.
The mechanism of specification of permanent cartilage is largely unknown. However, other investigators and we have reported that chondrocytes in permanent cartilage are able to express the terminal differentiation phenotype in vitro (Iwamoto et al. 1989; Pacifici et al. 1991; Stephens et al. 1992). In Cbfa1 transgenic mice, permanent cartilages such as articular cartilage, tracheal rings, nasal septum, and intervertebral disc underwent endochondral ossification. Taken together, it is likely that even permanent cartilage or cartilage fated to be permanent has the potential to be transient cartilage that enters endochondral pathway, and that lack of cell hypertrophy and matrix mineralization in permanent cartilage is due to negative regulation by microenvironmental cues and mechanisms, which could downregulate Cbfa1 expression. Degeneration of permanent cartilage is a feature of pathological change in osteoarthritis of the articular joints and hyperostosis of spine, such as ankylosis spondylitis or spondylosis of the spine (Sandell 1995). These diseases often displayed abnormal bone formation from cartilage, including subchondral bone sclerosis or osteophyte, associated with ectopic expression of several molecules such as type X collagen (von der Mark et al. 1992), osteopontin (Pullig et al. 2000), and matrix metalloproteinase 13 (MMP13) (Shlopov et al. 1997), which are normally specific to hypertrophic chondrocytes. Therefore, it has been proposed that the ossifying events in these diseases might be related to uncontrolled behavior of permanent chondrocytes and abnormal expression of hypertrophic phenotype. Ectopic ossification and ectopic expression of hypertrophic chondrocyte markers are characteristics of Cbfa1-transgenic mice. Further, Cbfa1 is able to induce the expression of osteopontin and MMP13 (Ducy et al. 1997; Komori et al. 1997; Shlopov et al. 1997; Sato et al. 1998; Harada et al. 1999; Inada et al. 1999; Jimenez et al. 1999; Porte et al. 1999). These findings suggest that Cbfa1 activation might be involved in permanent cartilage disorders. The mechanisms regulating Cbfa1 expression in chondrocytes are not yet fully clear and such information would provide important clues into cartilage development, including permanent cartilage organization, as well as the pathogenesis of osteoarthritis and spinal disorder.
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Acknowledgments |
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This work was supported by grants from the Ministry of Education, Science, and Culture, Japan, and the Tokyo Biochemical Research Foundation.
Submitted: 28 November 2000
Revised: 1 February 2001
Accepted: 2 February 2001
Abbreviations used in this paper: Cbfa1, core binding factor
1; Col2a1, 1 type II collagen; DN, dominant negative; GAPDH, glyceraldehyde-3-phosphate-dehydrogenase; GDF, growth and differentiation factor; H-E, hematoxylin and eosin; Ihh, Indian hedgehog; PTH, parathyroid hormone; PTHrP, PTH-related peptide; PTHrPR, PTHrP receptor.
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