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成釉细胞的分子与昼夜节律调控

Molecular and circadian controls of ameloblasts.

作者信息

Athanassiou-Papaefthymiou Maria, Kim Doohak, Harbron Lindsay, Papagerakis Silvana, Schnell Santiago, Harada Hidemitsu, Papagerakis Petros

机构信息

Department of Orthodontics and Pediatric Medicine, Center for Computational Medicine and Bioinformatics, University of Michigan Schools of Dentistry and Medicine, Ann Arbor, MI 48109, USA.

出版信息

Eur J Oral Sci. 2011 Dec;119 Suppl 1(Suppl 1):35-40. doi: 10.1111/j.1600-0722.2011.00918.x.

Abstract

Stage-specific expression of ameloblast-specific genes is controlled by differential expression of transcription factors. In addition, ameloblasts follow daily rhythms in their main activities (i.e. enamel protein secretion and enamel mineralization). This time-related control is orchestrated by oscillations of clock proteins involved in the regulation of circadian rhythms. Our aim was to identify the potential links between daily rhythms and developmental controls of ameloblast differentiation. The effects of the transcription factors distal-less homeobox 3 (Dlx3) and runt-related transcription factor 2 (Runx2), and the clock gene nuclear receptor subfamily 1, group D, member 1 (Nr1d1), on secretory and maturation ameloblasts [using stage-specific markers amelogenin (Amelx), enamelin (Enam), and kallikrein-related peptidase 4 (Klk4)] were evaluated in the HAT-7 ameloblast cell line. Amelx and Enam steady-state mRNA expression levels were down-regulated in Runx2 over-expressing cells and up-regulated in Dlx3 over-expressing cells. In contrast, Klk4 mRNA was up-regulated by both Dlx3 and Runx2. Furthermore, a temporal and spatial relationship between clock genes and ameloblast differentiation markers was detected. Of interest, clock genes not only affected rhythmic expression of ameloblast-specific genes but also influenced the expression of Runx2. Multiscale mathematical modeling is being explored to further understand the temporal and developmental controls of ameloblast differentiation. Our study provides novel insights into the regulatory mechanisms sustaining ameloblast differentiation.

摘要

成釉细胞特异性基因的阶段特异性表达受转录因子差异表达的控制。此外,成釉细胞在其主要活动(即釉质蛋白分泌和釉质矿化)中遵循每日节律。这种与时间相关的控制是由参与昼夜节律调节的时钟蛋白振荡协调的。我们的目的是确定每日节律与成釉细胞分化发育控制之间的潜在联系。在HAT-7成釉细胞系中评估了转录因子远端缺失同源盒3(Dlx3)和 runt相关转录因子2(Runx2)以及时钟基因核受体亚家族1 D组成员1(Nr1d1)对分泌性和成熟性成釉细胞[使用阶段特异性标志物釉原蛋白(Amelx)、釉蛋白(Enam)和激肽释放酶相关肽酶4(Klk4)]的影响。在Runx2过表达细胞中,Amelx和Enam的稳态mRNA表达水平下调,而在Dlx3过表达细胞中上调。相反,Klk4 mRNA在Dlx3和Runx2中均上调。此外,检测到时钟基因与成釉细胞分化标志物之间存在时间和空间关系。有趣的是,时钟基因不仅影响成釉细胞特异性基因的节律性表达,还影响Runx2的表达。正在探索多尺度数学模型以进一步了解成釉细胞分化的时间和发育控制。我们的研究为维持成釉细胞分化的调节机制提供了新的见解。

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