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无机磷酸盐对成牙骨质细胞基因表达的体外调控

Regulation of cementoblast gene expression by inorganic phosphate in vitro.

作者信息

Foster B L, Nociti F H, Swanson E C, Matsa-Dunn D, Berry J E, Cupp C J, Zhang P, Somerman M J

机构信息

Department of Periodontics, School of Dentistry, University of Washington, Seattle, WA, USA.

出版信息

Calcif Tissue Int. 2006 Feb;78(2):103-12. doi: 10.1007/s00223-005-0184-7. Epub 2006 Feb 6.

Abstract

Examination of mutant and knockout phenotypes with altered phosphate/pyrophosphate distribution has demonstrated that cementum, the mineralized tissue that sheathes the tooth root, is very sensitive to local levels of phosphate and pyrophosphate. The aim of this study was to examine the potential regulation of cementoblast cell behavior by inorganic phosphate (P(i)). Immortalized murine cementoblasts were treated with P(i) in vitro, and effects on gene expression (by quantitative real-time reverse-transcriptase polymerase chain reaction [RT-PCR]) and cell proliferation (by hemacytometer count) were observed. Dose-response (0.1-10 mM) and time-course (1-48 hours) assays were performed, as well as studies including the Na-P(i) uptake inhibitor phosphonoformic acid. Real-time RT-PCR indicated regulation by phosphate of several genes associated with differentiation/mineralization. A dose of 5 mM P(i) upregulated genes including the SIBLING family genes osteopontin (Opn, >300% of control) and dentin matrix protein-1 (Dmp-1, >3,000% of control). Another SIBLING family member, bone sialoprotein (Bsp), was downregulated, as were osteocalcin (Ocn) and type I collagen (Col1). Time-course experiments indicated that these genes responded within 6-24 hours. Time-course experiments also indicated rapid regulation (by 6 hours) of genes concerned with phosphate/pyrophosphate homeostasis, including the mouse progressive ankylosis gene (Ank), plasma cell membrane glycoprotein-1 (Pc-1), tissue nonspecific alkaline phosphatase (Tnap), and the Pit1 Na-P(i) cotransporter. Phosphate effects on cementoblasts were further shown to be uptake-dependent and proliferation-independent. These data suggest regulation by phosphate of multiple genes in cementoblasts in vitro. During formation, phosphate and pyrophosphate may be important regulators of cementoblast functions including maturation and regulation of matrix mineralization.

摘要

对具有改变的磷酸盐/焦磷酸盐分布的突变体和基因敲除表型进行的研究表明,牙骨质(包裹牙根的矿化组织)对局部磷酸盐和焦磷酸盐水平非常敏感。本研究的目的是研究无机磷酸盐(P(i))对成牙骨质细胞行为的潜在调节作用。将永生化小鼠成牙骨质细胞在体外用P(i)处理,并观察其对基因表达(通过定量实时逆转录聚合酶链反应[RT-PCR])和细胞增殖(通过血细胞计数器计数)的影响。进行了剂量反应(0.1-10 mM)和时间进程(1-48小时)试验,以及包括Na-P(i)摄取抑制剂膦甲酸的研究。实时RT-PCR表明磷酸盐对与分化/矿化相关的几个基因有调节作用。5 mM P(i)的剂量上调了包括SIBLING家族基因骨桥蛋白(Opn,>对照的300%)和牙本质基质蛋白-1(Dmp-1,>对照的3000%)在内的基因。另一个SIBLING家族成员骨唾液蛋白(Bsp)以及骨钙素(Ocn)和I型胶原(Col1)被下调。时间进程实验表明这些基因在6-24小时内做出反应。时间进程实验还表明与磷酸盐/焦磷酸盐稳态相关的基因(包括小鼠进行性关节强硬基因[Ank]、浆细胞膜糖蛋白-1[Pc-1]、组织非特异性碱性磷酸酶[Tnap]和Pit1 Na-P(i)共转运体)在6小时内迅速受到调节。磷酸盐对成牙骨质细胞的影响进一步表明是摄取依赖性的且与增殖无关。这些数据表明体外磷酸盐对成牙骨质细胞中的多个基因有调节作用。在形成过程中,磷酸盐和焦磷酸盐可能是成牙骨质细胞功能(包括成熟和基质矿化调节)的重要调节因子。

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