Yamashiro Takashi, Wang Xiu-Ping, Li Zhe, Oya Shinji, Aberg Thomas, Fukunaga Tomohiro, Kamioka Hiroshi, Speck Nancy A, Takano-Yamamoto Teruko, Thesleff Irma
Department of Orthodontics, Graduate School of Medicine and Dentistry, Okayama University, Okayama, Japan.
J Bone Miner Res. 2004 Oct;19(10):1671-7. doi: 10.1359/JBMR.040801. Epub 2004 Aug 3.
We evaluated the detailed expression patterns of Runx1 and Sox9 in various types of bone formation, and determined whether Runx1 expression was affected by Runx2 deficiency and Runx2 expression by Runx1 deficiency. Our results indicate that both Runx1 and Sox9 are intensely expressed in the future osteogenic cell compartment and in cartilage. The pattern of Runx1 and Sox9 expression suggests that both genes could potentially be involved in incipient intramembranous bone formation during craniofacial development.
Runx1, a gene essential for hematopoiesis, contains RUNX binding sites in its promoter region, suggesting possible cross-regulation with Runx2 and potential regulatory roles in bone development. On the other hand, Sox9 is essential for chondrogenesis, and haploinsufficiency of Sox9 leads to premature ossification of the skeletal system. In this study, we studied the possible roles of Runx1 and Sox9 in bone development.
Runx1, Runx2/Osf2, and Sox9 expression was evaluated by in situ hybridization in the growing craniofacial bones of embryonic day (E)12-16 mice and in the endochondral bone-forming regions of embryonic and postnatal long bones. In addition, we evaluated Runx2/Osf2 expression in the growing face of Runx1 knockout mice at E12.5 and Runx1 expression in Runx2 knockout mice at E14.5.
Runx1 and Sox9 were expressed in cartilage, and the regions of expression expanded to the neighboring Runx2-expressing osteogenic regions. Expression of both Runx1 and Sox9 was markedly downregulated on ossification. Runx1 and Sox9 expression was absent in the regions of endochondral bone formation and in actively modeling or remodeling bone tissues in the long bones as well as in ossified craniofacial bones. Runx2 expression was not affected by gene disruption of Runx1, whereas the expression domains of Runx1 were extended in Runx2(-/-) mice compared with wildtype mice.
Runx1 and Sox9 are specifically expressed in the osteogenic cell compartments in the craniofacial bones and the bone collar of long bones, and this expression is downregulated on terminal differentiation of osteoblasts. Our results suggest that Runx1 may play a role in incipient intramembranous bone formation.
我们评估了Runx1和Sox9在各种类型骨形成中的详细表达模式,并确定Runx1的表达是否受Runx2缺陷的影响以及Runx2的表达是否受Runx1缺陷的影响。我们的结果表明,Runx1和Sox9在未来的成骨细胞区室和软骨中均强烈表达。Runx1和Sox9的表达模式表明这两个基因可能都参与颅面发育过程中初期的膜内骨形成。
Runx1是造血必需基因,其启动子区域含有RUNX结合位点,提示可能与Runx2存在交叉调节以及在骨发育中具有潜在调节作用。另一方面,Sox9对软骨形成至关重要,Sox9单倍剂量不足会导致骨骼系统过早骨化。在本研究中,我们研究了Runx1和Sox9在骨发育中的可能作用。
通过原位杂交评估胚胎第(E)12 - 16天小鼠生长中的颅面骨以及胚胎和出生后长骨的软骨内骨形成区域中Runx1、Runx2/Osf2和Sox9的表达。此外,我们评估了E12.5时Runx1基因敲除小鼠生长面部中Runx2/Osf2的表达以及E14.5时Runx2基因敲除小鼠中Runx1的表达。
Runx1和Sox9在软骨中表达,且表达区域扩展至邻近的表达Runx2的成骨区域。在骨化时,Runx1和Sox9的表达均明显下调。在软骨内骨形成区域以及长骨中正在进行塑形或重塑的骨组织以及骨化的颅面骨中,Runx1和Sox9均无表达。Runx2的表达不受Runx1基因破坏的影响,而与野生型小鼠相比,Runx1的表达域在Runx2(-/-)小鼠中有所扩展。
Runx1和Sox9在颅面骨和成骨细胞区室以及长骨的骨环中特异性表达,且在成骨细胞终末分化时该表达下调。我们的结果提示Runx1可能在初期的膜内骨形成中发挥作用。
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