Osteoblast differentiation of Gli1⁺ cells via Wnt and BMP signaling pathways during orthodontic tooth movement

IF 2.6 Q1 DENTISTRY, ORAL SURGERY & MEDICINE Journal of Oral Biosciences Pub Date : 2024-06-01 DOI:10.1016/j.job.2024.03.004
Yuri Seki , Hiroaki Takebe , Yuya Nakao , Kohei Sato , Toshihide Mizoguchi , Hiroaki Nakamura , Masahiro Iijima , Akihiro Hosoya
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引用次数: 0

Abstract

Objectives

Factors that induce bone formation during orthodontic tooth movement (OTM) remain unclear. Gli1 was recently identified as a stem cell marker in the periodontal ligament (PDL). Therefore, we evaluated the mechanism of differentiation of Cre/LoxP-mediated Gli1/Tomato+ cells into osteoblasts during OTM.

Methods

After the final administration of tamoxifen to 8-week-old Gli1-CreERT2/ROSA26-loxP-stop-loxP-tdTomato mice for 2 days, nickel–titanium closed coil springs were attached between the upper anterior alveolar bone and the first molar. Immunohistochemical localizations of β-catenin, Smad4, and Runx2 were observed in the PDL on 2, 5, and 10 days after OTM initiation.

Results

In the untreated tooth, few Gli1/Tomato+ cells were detected in the PDL. Two days after OTM initiation, the number of Gli1/Tomato+ cells increased in the PDL on the tension side. On this side, 49.3 ± 7.0% of β-catenin+ and 48.7 ± 5.7% of Smad4+ cells were found in the PDL, and Runx2 expression was detected in some Gli1/Tomato+ cells apart from the alveolar bone. The number of positive cells in the PDL reached a maximum on day 5. In contrast, on the compression side, β-catenin and Smad4 exhibited less immunoreactivity. On day 10, Gli1/Tomato+ cells were aligned on the alveolar bone on the tension side, with some expressing Runx2.

Conclusions

Gli1+ cells in the PDL differentiated into osteoblasts during OTM. Wnt and bone morphogenetic proteins signaling pathways may be involved in this differentiation.

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在牙齿矫正过程中,Gli1⁺细胞通过 Wnt 和 BMP 信号通路进行成骨细胞分化。
目的:正畸牙齿移动(OTM)过程中诱导骨形成的因素仍不清楚。最近发现 Gli1 是牙周韧带 (PDL) 中的干细胞标记。因此,我们评估了OTM期间Cre/LoxP介导的Gli1/Tomato+细胞向成骨细胞分化的机制:方法:给 8 周龄的 Gli1-CreERT2/ROSA26-loxP-stop-loxP-tdTomato 小鼠注射他莫昔芬 2 天后,在上前牙槽骨和第一磨牙之间连接镍钛闭合螺旋弹簧。结果显示:在OTM开始后的2天、5天和10天,在PDL中观察了β-catenin、Smad4和Runx2的免疫组化定位:结果:在未处理的牙齿中,PDL 中检测到少量 Gli1/Tomato+ 细胞。开始 OTM 两天后,张力侧 PDL 中 Gli1/Tomato+ 细胞数量增加。在这一侧,PDL中发现了49.3±7.0%的β-catenin+细胞和48.7±5.7%的Smad4+细胞,在除牙槽骨外的一些Gli1/Tomato+细胞中检测到了Runx2的表达。PDL 中阳性细胞的数量在第 5 天达到最大值。相比之下,在压迫侧,β-catenin 和 Smad4 的免疫活性较低。第10天,Gli1/Tomato+细胞排列在张力侧的牙槽骨上,部分细胞表达Runx2:结论:PDL中的Gli1+细胞在OTM过程中分化为成骨细胞。结论:PDL中的Gli1+细胞在OTM过程中分化为成骨细胞,Wnt和骨形态发生蛋白信号通路可能参与了这种分化。
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来源期刊
Journal of Oral Biosciences
Journal of Oral Biosciences DENTISTRY, ORAL SURGERY & MEDICINE-
CiteScore
4.40
自引率
12.50%
发文量
57
审稿时长
37 days
期刊最新文献
Editorial Board Oral microbiome profiles of gingivitis and periodontitis by next-generation sequencing among a group of hospital patients in Korea: A cross-sectional study. Exploring the Mechanism of tiRNA-Val-CAC-002 in the Pathogenesis of Oral Submucous Fibrosis. Impact of organic, conventional, and stingless bee honeys on the antibacterial activity of gummy candies against oral bacteria. CCN2: a potential contributor to gingival overgrowth.
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