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Mast4 决定了间充质干细胞向成骨细胞和软骨细胞分化的命运。

Mast4 determines the cell fate of MSCs for bone and cartilage development.

机构信息

GILO Institute, GILO Foundation, Seoul, 06668, Korea.

Department of Biomedical Science, College of Life Science, CHA University, Seongnam City, 463-400, Kyunggi-do, Korea.

出版信息

Nat Commun. 2022 Jul 8;13(1):3960. doi: 10.1038/s41467-022-31697-3.

Abstract

Mesenchymal stromal cells (MSCs) differentiation into different lineages is precisely controlled by signaling pathways. Given that protein kinases play a crucial role in signal transduction, here we show that Microtubule Associated Serine/Threonine Kinase Family Member 4 (Mast4) serves as an important mediator of TGF-β and Wnt signal transduction in regulating chondro-osteogenic differentiation of MSCs. Suppression of Mast4 by TGF-β1 led to increased Sox9 stability by blocking Mast4-induced Sox9 serine 494 phosphorylation and subsequent proteasomal degradation, ultimately enhancing chondrogenesis of MSCs. On the other hand, Mast4 protein, which stability was enhanced by Wnt-mediated inhibition of GSK-3β and subsequent Smurf1 recruitment, promoted β-catenin nuclear localization and Runx2 activity, increasing osteogenesis of MSCs. Consistently, Mast4 mice demonstrated excessive cartilage synthesis, while exhibiting osteoporotic phenotype. Interestingly, Mast4 depletion in MSCs facilitated cartilage formation and regeneration in vivo. Altogether, our findings uncover essential roles of Mast4 in determining the fate of MSC development into cartilage or bone.

摘要

间充质基质细胞(MSCs)向不同谱系的分化受到信号通路的精确控制。鉴于蛋白激酶在信号转导中起着至关重要的作用,我们在此表明微管相关丝氨酸/苏氨酸激酶家族成员 4(Mast4)在调节 MSC 的软骨 - 成骨分化中作为 TGF-β 和 Wnt 信号转导的重要介质。TGF-β1 通过抑制 Mast4 诱导的 Sox9 丝氨酸 494 磷酸化和随后的蛋白酶体降解来抑制 Mast4,从而导致 Sox9 稳定性增加,最终增强了 MSC 的软骨生成。另一方面,Mast4 蛋白的稳定性通过 Wnt 介导的 GSK-3β抑制和随后的 Smurf1 募集得到增强,促进了 β-连环蛋白的核定位和 Runx2 活性,从而增加了 MSC 的成骨作用。一致地,Mast4 敲除小鼠表现出过度的软骨合成,同时表现出骨质疏松表型。有趣的是,MSC 中 Mast4 的耗竭促进了体内软骨的形成和再生。总的来说,我们的研究结果揭示了 Mast4 在决定 MSC 向软骨或骨发育命运中的重要作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e955/9270402/939f265d6355/41467_2022_31697_Fig1_HTML.jpg

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