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胰岛素受体底物-1在胰岛素样生长因子-I介导的骨髓间充质干细胞软骨生成性增殖、分化和肥大中的亚细胞定位

Subcellular localization of IRS-1 in IGF-I-mediated chondrogenic proliferation, differentiation and hypertrophy of bone marrow mesenchymal stem cells.

作者信息

Longobardi Lara, Granero-Moltó Froilán, O'Rear Lynda, Myers Timothy J, Li Tieshi, Kregor Philip J, Spagnoli Anna

机构信息

Department of Pediatrics, University of North Carolina at Chapel Hill, Chapel Hill, NC 27599-7039, USA.

出版信息

Growth Factors. 2009 Oct;27(5):309-20. doi: 10.1080/08977190903138874.

DOI:10.1080/08977190903138874
PMID:19639489
Abstract

Bone marrow derived mesenchymal stem cells (BM-MSC) can differentiate into chondrocytes. Understanding the mechanisms and growth factors that control the MSC stemness is critical to fully implement their therapeutic use in cartilage diseases. The activated type 1 insulin-like growth factor receptor (IGF-IR), interacting with the insulin receptor substrate-1 (IRS-1), can induce cancer cell proliferation and transformation. In cancer or transformed cells, IRS-1 has been shown to localize in the cytoplasm where it activates the canonical Akt pathway, as well as in the nucleus where it binds to nuclear proteins. We have previously demonstrated that IGF-I has distinct time-dependent effect on primary BM-MSC chondrogenic pellets: initially (2-day culture), IGF-I induces proliferation; subsequently, IGF-I promotes chondrocytic differentiation (7-day culture). In the present study, by using MSC from the BM of IRS-1(- / - ) mice we show that IRS-1 mediates almost 50% of the IGF-I mitogenic response and the MAPK-MEK/ERK signalling accounts for the other 50%. After stimulation with IGF-I, we found that in 2-day old human and mouse derived BM-MSC pellets, IRS-1 (total and phosphorylated) is nuclearly localized and that proliferation prevails over differentiation. The IGF-I mitogenic effect is Akt-independent. In 7-day MSC pellets, IGF-I stimulates the chondrogenic differentiation of MSC into chondrocytes, pre-hypertrophic and hypertrophic chondrocytes and IRS-1 accumulates in the cytoplasm. IGF-I-dependent differentiation is exclusively Akt-dependent. Our data indicate that in the physiologically relevant model of primary cultured MSC, IGF-I induces a temporally regulated nuclear or cytoplasmic localization of IRS-1 that correlate with the transition from proliferation to chondrogenic differentiation.

摘要

骨髓间充质干细胞(BM-MSC)可分化为软骨细胞。了解控制MSC干性的机制和生长因子对于在软骨疾病中充分发挥其治疗作用至关重要。激活的1型胰岛素样生长因子受体(IGF-IR)与胰岛素受体底物-1(IRS-1)相互作用,可诱导癌细胞增殖和转化。在癌细胞或转化细胞中,IRS-1已被证明定位于细胞质中,在那里它激活经典的Akt途径,以及定位于细胞核中,在那里它与核蛋白结合。我们之前已经证明IGF-I对原代BM-MSC软骨生成微球有明显的时间依赖性影响:最初(2天培养),IGF-I诱导增殖;随后,IGF-I促进软骨细胞分化(7天培养)。在本研究中,通过使用来自IRS-1(- / -)小鼠骨髓的MSC,我们发现IRS-1介导了近50%的IGF-I促有丝分裂反应,而MAPK-MEK/ERK信号传导则占另外50%。用IGF-I刺激后,我们发现在2天大的人和小鼠来源的BM-MSC微球中,IRS-1(总蛋白和磷酸化蛋白)定位于细胞核,且增殖胜过分化。IGF-I的促有丝分裂作用不依赖于Akt。在7天的MSC微球中,IGF-I刺激MSC向软骨细胞、前肥大软骨细胞和肥大软骨细胞分化,且IRS-1在细胞质中积累。IGF-I依赖性分化完全依赖于Akt。我们的数据表明,在原代培养的MSC的生理相关模型中,IGF-I诱导IRS-1在时间上受到调节的核或细胞质定位,这与从增殖到软骨生成分化的转变相关。

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