YBX1促进牙髓干细胞中RUNX2替代外显子5的包含。

IF 2.5 4区 医学 Q3 CELL & TISSUE ENGINEERING International journal of stem cells Pub Date : 2022-08-30 Epub Date: 2021-12-31 DOI:10.15283/ijsc21035
Jiaoxiang Shen, Wenting She, Fengxia Zhang, Jihua Guo, Rong Jia
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引用次数: 1

摘要

背景与目的:RUNX2在牙髓干细胞(dental pulp stem cells, DPSCs)成牙细胞分化过程中起重要作用。RUNX2外显子5是另一个外显子,对RUNX2的转录活性至关重要。本研究旨在探讨RUNX2外显子5选择性剪接在人DPSCs中的调控机制。方法和结果:使用在线SpliceAid程序分析RUNX2外显子5的调控基序。RT-PCR分析了矿化诱导DPSCs分化过程中RUNX2外显子5的选择性剪接。为了探讨剪接因子YBX1对5外显子选择性剪接的影响,在DPSCs中通过转染YBX1过表达质粒或抗YBX1 siRNA来获得或失去YBX1的功能。人类RUNX2外显子5在进化上是保守的,并且在DPSCs中有选择性剪接。RUNX2外显子5中有三个潜在的YBX1结合基序。在矿化诱导的DPSCs分化过程中,RUNX2外显子5和YBX1的表达水平显著升高。YBX1过表达显著增加了RUNX2外显子5在DPSCs中的表达。相比之下,YBX1的沉默显著降低了5外显子的内含以及相应的RUNX2蛋白表达水平。YBX1基因敲低可降低碱性磷酸酶(ALP)和骨钙素(OC)的表达,降低DPSCs的矿化能力,而YBX1基因过表达可提高ALP和OC的表达,提高DPSCs的矿化能力。结论:人类RUNX2外显子5在进化上是保守的,并且在DPSCs中具有选择性剪接。剪接因子YBX1促进RUNX2外显子5的包合,提高DPSCs的矿化能力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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YBX1 Promotes the Inclusion of RUNX2 Alternative Exon 5 in Dental Pulp Stem Cells.

Background and objectives: RUNX2 plays an essential role during the odontoblast differentiation of dental pulp stem cells (DPSCs). RUNX2 Exon 5 is an alternative exon and essential for RUNX2 transcriptional activity. This study aimed to investigate the regulatory mechanisms of RUNX2 exon 5 alternative splicing in human DPSCs.

Methods and results: The regulatory motifs of RUNX2 exon 5 were analyzed using the online SpliceAid program. The alternative splicing of RUNX2 exon 5 in DPSCs during mineralization-induced differentiation was analyzed by RT-PCR. To explore the effect of splicing factor YBX1 on exon 5 alternative splicing, gaining or losing function of YBX1 was performed by transfection of YBX1 overexpression plasmid or anti-YBX1 siRNA in DPSCs. Human RUNX2 exon 5 is evolutionarily conserved and alternatively spliced in DPSCs. There are three potential YBX1 binding motifs in RUNX2 exon 5. The inclusion of RUNX2 exon 5 and YBX1 expression level increased significantly during mineralization- induced differentiation in DPSCs. Overexpression of YBX1 significantly increased the inclusion of RUNX2 exon 5 in DPSCs. In contrast, silence of YBX1 significantly reduced the inclusion of exon 5 and the corresponding RUNX2 protein expression level. Knockdown of YBX1 reduced the expression of alkaline phosphatase (ALP) and osteocalcin (OC) and the mineralization ability of DPSCs, while overexpression of YBX1 increased the expression of ALP and OC and the mineralization ability of DPSCs.

Conclusions: Human RUNX2 exon 5 is conserved evolutionarily and alternatively spliced in DPSCs. Splicing factor YBX1 promotes the inclusion of RUNX2 exon 5 and improves the mineralization ability of DPSCs.

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来源期刊
International journal of stem cells
International journal of stem cells Biochemistry, Genetics and Molecular Biology-Cell Biology
CiteScore
5.10
自引率
4.30%
发文量
38
期刊介绍: International Journal of Stem Cells (Int J Stem Cells), a peer-reviewed open access journal, principally aims to provide a forum for investigators in the field of stem cell biology to present their research findings and share their visions and opinions. Int J Stem Cells covers all aspects of stem cell biology including basic, clinical and translational research on genetics, biochemistry, and physiology of various types of stem cells including embryonic, adult and induced stem cells. Reports on epigenetics, genomics, proteomics, metabolomics of stem cells are welcome as well. Int J Stem Cells also publishes review articles, technical reports and treatise on ethical issues.
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