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Smoc1 和 Smoc2 作为 Runx2 的下游分子调节骨形成。

Smoc1 and Smoc2 regulate bone formation as downstream molecules of Runx2.

机构信息

Department of Molecular and Cellular Biochemistry, Osaka University Graduate School of Dentistry, Osaka, Japan.

Laboratory for Animal Resources and Genetic Engineering, RIKEN Center for Biosystems Dynamics Research, Hyogo, Japan.

出版信息

Commun Biol. 2021 Oct 19;4(1):1199. doi: 10.1038/s42003-021-02717-7.

Abstract

Runx2 is an essential transcription factor for bone formation. Although osteocalcin, osteopontin, and bone sialoprotein are well-known Runx2-regulated bone-specific genes, the skeletal phenotypes of knockout (KO) mice for these genes are marginal compared with those of Runx2 KO mice. These inconsistencies suggest that unknown Runx2-regulated genes play important roles in bone formation. To address this, we attempted to identify the Runx2 targets by performing RNA-sequencing and found Smoc1 and Smoc2 upregulation by Runx2. Smoc1 or Smoc2 knockdown inhibited osteoblastogenesis. Smoc1 KO mice displayed no fibula formation, while Smoc2 KO mice had mild craniofacial phenotypes. Surprisingly, Smoc1 and Smoc2 double KO (DKO) mice manifested no skull, shortened tibiae, and no fibulae. Endochondral bone formation was also impaired at the late stage in the DKO mice. Collectively, these results suggest that Smoc1 and Smoc2 function as novel targets for Runx2, and play important roles in intramembranous and endochondral bone formation.

摘要

Runx2 是成骨所必需的转录因子。尽管骨钙素、骨桥蛋白和骨涎蛋白是众所周知的受 Runx2 调控的骨特异性基因,但这些基因敲除(KO)小鼠的骨骼表型与 Runx2 KO 小鼠相比微不足道。这些不一致表明,未知的受 Runx2 调控的基因在骨形成中发挥着重要作用。为了解决这个问题,我们试图通过 RNA 测序来鉴定 Runx2 的靶基因,并发现 Smoc1 和 Smoc2 受 Runx2 上调。Smoc1 或 Smoc2 的敲低抑制成骨细胞的生成。Smoc1 KO 小鼠的腓骨没有形成,而 Smoc2 KO 小鼠则表现出轻微的颅面表型。令人惊讶的是,Smoc1 和 Smoc2 双敲除(DKO)小鼠则没有颅骨,胫骨缩短,没有腓骨。在 DKO 小鼠中晚期也出现了软骨内骨形成受损的情况。总的来说,这些结果表明 Smoc1 和 Smoc2 作为 Runx2 的新型靶基因,在膜内和软骨内骨形成中发挥重要作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b195/8526618/4ed4d7a34e9a/42003_2021_2717_Fig1_HTML.jpg

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