mettl1介导的tRNA m7G修饰通过p53信号调控牙根发育过程中牙本质的形成。

IF 5.9 1区医学 Q1 ENDOCRINOLOGY & METABOLISM

Journal of Bone and Mineral Research Pub Date : 2025-06-03 DOI:10.1093/jbmr/zjaf056

Xinyan Gan, Kun He, Qiuchan Xiong, Rui Sheng, Kexin Lei, Shuang Jiang, Xiaoyu Yang, Yimeng Cai, Denghao Huang, Yu Shi, Ling Ye, Quan Yuan, Qiwen Li

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引用次数: 0

摘要

tRNA n7 -甲基鸟苷（m7G）是哺乳动物中最丰富的表观遗传修饰之一，它是由甲基转移酶1-WD重复蛋白4 （METTL1-WDR4）复合物催化的。WDR4的错义突变与原始侏儒症有关，后者表现出严重的颅面发育畸形，包括小牙齿，但其潜在的分子机制仍不清楚。在本研究中，我们探讨了m7G修饰对牙根发育过程中牙本质形成的影响。METTL1在小鼠牙根发育过程中表达活跃，在牙根形成后无法检测到其表达。接下来，我们生成Prrx1-Cre驱动的Mettl1 （Prrx1Cre;Mettl1fl/fl）条件敲除小鼠，删除牙间质中Mettl1，并探讨其在牙齿发育过程中的调控作用。显微计算机断层扫描显示，与同窝对照相比，Prrx1Cre；Mettl1fl/fl小鼠下颌第一磨牙的牙根更短、更小，牙根区域和冠区域的牙本质和前牙本质的宽度都减少了。Wdr4R215L/R215L小鼠也表现出牙根缩短和牙本质变薄，与Prrx1Cre；Mettl1fl/fl小鼠表型相似。此外，mettl1缺失的人牙髓细胞（hDPCs）的增殖、迁移和成牙分化能力下降。RNA-seq显示Mettl1缺失后p53信号通路上调和细胞周期阻滞。PFT-α（一种p53信号抑制剂）可以部分挽救mettl1缺失的hDPCs的增殖和牙源性分化。综上所述，我们的研究结果表明，mettl1介导的tRNA m7G修饰缺失会通过p53信号通路损害hDPCs的增殖和成牙分化，并影响牙根发育过程中牙本质的形成，为小牙提供了一种新的表观遗传机制。

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Methyltransferase 1-mediated tRNA N7-methylguanosine modification regulates dentin formation during tooth root development via p53 signaling.

tRNA N7-methylguanosine (m7G) is one of the most abundant epigenetic modifications in mammals, which is catalyzed by the methyltransferase 1-WD repeat-containing protein 4 (METTL1-WDR4) complex. Missense mutations in WDR4 have been linked to primordial dwarfism, which shows severe craniofacial developmental deformities including small teeth, but the underlying molecular mechanisms remain elusive. In this study, we explore the effect of m7G modification on dentin formation during tooth root development. METTL1 was actively expressed in mice developing tooth roots, and its expression became undetectable after tooth root formation. Next, we generated Prrx1-Cre driven Mettl1 (Prrx1Cre;Mettl1fl/fl) conditional KO mice to delete Mettl1 in dental mesenchyme and explored its regulation during tooth development. Micro-computed tomography revealed that the roots of the mandibular first molar in Prrx1Cre;Mettl1fl/fl mice were shorter and smaller compared to littermate control, with a reduction in the width of dentin and pre-dentin in both the root area and the crown area. Wdr4R215L/R215L mice also exhibited tooth root shortening and dentin thinning, phenocopying the Prrx1Cre;Mettl1fl/fl mice. Moreover, METTL1-depleted human dental pulp cells (hDPCs) showed decreased ability of proliferation, migration, and odontogenic differentiation. RNA-seq revealed upregulation of the p53 signaling pathway and cell cycle arrest after deletion of Mettl1. The proliferation and odontogenic differentiation of METTL1-depleted hDPCs is partially rescued with pifithrin-α (PFT-α), a p53 signaling inhibitor. Taken together, our results demonstrate that loss of METTL1-mediated tRNA m7G modification impairs the proliferation and odontogenic differentiation of hDPCs via the p53 signaling pathway and affects the dentin formation during tooth root development, providing a novel epigenetic mechanism underlying small teeth.

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来源期刊

Journal of Bone and Mineral Research 医学-内分泌学与代谢

CiteScore

11.30

自引率

6.50%

发文量

257

审稿时长

2 months

期刊介绍： The Journal of Bone and Mineral Research (JBMR) publishes highly impactful original manuscripts, reviews, and special articles on basic, translational and clinical investigations relevant to the musculoskeletal system and mineral metabolism. Specifically, the journal is interested in original research on the biology and physiology of skeletal tissues, interdisciplinary research spanning the musculoskeletal and other systems, including but not limited to immunology, hematology, energy metabolism, cancer biology, and neurology, and systems biology topics using large scale “-omics” approaches. The journal welcomes clinical research on the pathophysiology, treatment and prevention of osteoporosis and fractures, as well as sarcopenia, disorders of bone and mineral metabolism, and rare or genetically determined bone diseases.