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骨桥蛋白在机械应力引起的骨重塑中的作用。

Role of osteopontin in bone remodeling caused by mechanical stress.

作者信息

Terai K, Takano-Yamamoto T, Ohba Y, Hiura K, Sugimoto M, Sato M, Kawahata H, Inaguma N, Kitamura Y, Nomura S

机构信息

Department of Orthodontics, Tokushima University School of Dentistry, Tokushima, Japan.

出版信息

J Bone Miner Res. 1999 Jun;14(6):839-49. doi: 10.1359/jbmr.1999.14.6.839.

DOI:10.1359/jbmr.1999.14.6.839
PMID:10352091
Abstract

Changes in the number and proportion of osteopontin mRNA (Opn) expressing osteocytes and osteoclasts caused by the mechanical stress applied during experimental tooth movement were examined in the present study. Opn expression was detected in the osteocytes on the pressure side at the early stage, and gradually spread to those on the tension side and also to the osteoblasts and bone-lining cells in the alveolar bone. Only 3.3% of the osteocytes located on the pressure side expressed Opn in the interradicular septum of control rats; in contrast, the value was increased to 87.5% at 48 h after the initiation of tooth movement. These results indicate that these cells responded to mechanical stress loaded on the bone with expression of the osteopontin gene. Following the increased expression of Opn in these cells, a 17-fold greater number of osteoclasts compared with the control and numerous resorption pits were observed on the pressure side of the alveolar bone. Injection of arginine-glycine-aspartic acid-serine peptide but not that of arginine-glycine-glutamic acid-serine peptide strongly inhibited the increase in the number of osteoclasts. Furthermore, an in vitro migration assay demonstrated the chemotactic activity of osteopontin (OPN) on the precursor of osteoclasts. Our study strongly suggests that OPN is an important factor triggering bone remodeling caused by mechanical stress.

摘要

在本研究中,检测了实验性牙齿移动过程中施加的机械应力所引起的表达骨桥蛋白mRNA(Opn)的骨细胞和破骨细胞数量及比例的变化。在早期,压力侧的骨细胞中检测到Opn表达,并逐渐扩散到张力侧的骨细胞以及牙槽骨中的成骨细胞和骨衬细胞。在对照大鼠的根间间隔中,位于压力侧的骨细胞仅有3.3%表达Opn;相比之下,在牙齿移动开始后48小时,该值增加到了87.5%。这些结果表明,这些细胞通过骨桥蛋白基因的表达对施加在骨上的机械应力作出反应。在这些细胞中Opn表达增加后,与对照组相比,在牙槽骨压力侧观察到破骨细胞数量增加了17倍,并且有大量的吸收陷窝。注射精氨酸 - 甘氨酸 - 天冬氨酸 - 丝氨酸肽而非精氨酸 - 甘氨酸 - 谷氨酸 - 丝氨酸肽可强烈抑制破骨细胞数量的增加。此外,体外迁移试验证明了骨桥蛋白(OPN)对破骨细胞前体的趋化活性。我们的研究强烈表明,OPN是引发机械应力导致骨重塑的重要因素。

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