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氢氧化钙通过 CEMP1 和 ERK 依赖性途径促进骨形成和诱导间充质牙周膜细胞的成牙骨质分化。

Calcium hydroxide promotes cementogenesis and induces cementoblastic differentiation of mesenchymal periodontal ligament cells in a CEMP1- and ERK-dependent manner.

机构信息

Department of Periodontics and Oral Medicine, School of Dentistry, University of Michigan, 1011 N. University Ave., Ann Arbor, MI 48109-1078, USA.

出版信息

Calcif Tissue Int. 2010 Aug;87(2):144-57. doi: 10.1007/s00223-010-9368-x. Epub 2010 May 4.

DOI:10.1007/s00223-010-9368-x
PMID:20440482
Abstract

Periodontal tissue engineering is a complex process requiring the regeneration of bone, cementum, and periodontal ligament (PDL). Since cementum regeneration is poorly understood, we used a dog model of dental pulpal necrosis and in vitro cellular wounding and mineralization assays to determine the mechanism of action of calcium hydroxide, Ca(OH)(2), in cementogenesis. Laser capture microdissection (LCM) followed by qRT-PCR were used to assay responses of periapical tissues to Ca(OH)(2) treatment. Additionally, viability, proliferation, migration, and mineralization responses of human mesenchymal PDL cells to Ca(OH)(2) were assayed. Finally, biochemical inhibitors and siRNA were used to investigate Ca(OH)(2)-mediated signaling in PDL cell differentiation. In vivo, Ca(OH)(2)-treated teeth formed a neocementum in a STRO-1- and cementum protein-1 (CEMP1)-positive cellular environment. LCM-harvested tissues adjacent to the neocementum exhibited higher mRNA levels for CEMP1, integrin-binding sialoprotein, and Runx2 than central PDL cells. In vitro, Ca(OH)(2) and CEMP1 promoted STRO-1-positive cell proliferation, migration, and wound closure. Ca(OH)(2) stimulated expression of the cementum-specific proteins CEMP1 and PTPLA/CAP in an ERK-dependent manner. Lastly, Ca(OH)(2) stimulated mineralization by CEMP1-positive cells. Blocking CEMP1 and ERK function abolished Ca(OH)(2)-induced mineralization, confirming a role for CEMP1 and ERK in the process. Ca(OH)(2) promotes cementogenesis and recruits STRO-1-positive mesenchymal PDL cells to undergo cementoblastic differentiation and mineralization via a CEMP1- and ERK-dependent pathway.

摘要

牙周组织工程是一个复杂的过程,需要再生骨、牙骨质和牙周膜(PDL)。由于牙骨质再生的机制尚未完全了解,我们使用狗牙髓坏死模型和体外细胞损伤和矿化测定来确定氢氧化钙(Ca(OH)(2))在牙骨质形成中的作用机制。采用激光捕获显微切割(LCM)联合 qRT-PCR 检测根尖组织对 Ca(OH)(2)处理的反应。此外,还检测了人骨髓间充质 PDL 细胞对 Ca(OH)(2)的活力、增殖、迁移和矿化反应。最后,使用生化抑制剂和 siRNA 研究了 Ca(OH)(2)介导的 PDL 细胞分化信号通路。在体内,用 Ca(OH)(2)处理的牙齿在 STRO-1 和牙骨质蛋白 1(CEMP1)阳性细胞环境中形成新生牙骨质。与新生牙骨质相邻的 LCM 采集组织的 CEMP1、整合素结合唾液蛋白和 Runx2 的 mRNA 水平高于中央 PDL 细胞。在体外,Ca(OH)(2)和 CEMP1 促进 STRO-1 阳性细胞增殖、迁移和伤口闭合。Ca(OH)(2)以 ERK 依赖的方式刺激牙骨质特异性蛋白 CEMP1 和 PTPLA/CAP 的表达。最后,CEMP1 阳性细胞通过 Ca(OH)(2)刺激矿化。阻断 CEMP1 和 ERK 功能可消除 Ca(OH)(2)诱导的矿化,证实 CEMP1 和 ERK 在该过程中起作用。Ca(OH)(2)通过 CEMP1 和 ERK 依赖途径促进牙骨质形成,并募集 STRO-1 阳性间充质 PDL 细胞向牙骨质母细胞分化和矿化。

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