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短发夹 RNA 下调 PKD1 通过 cAMP/PKA 通路导致人 MG-63 细胞成骨分化缺陷。

Downregulation of PKD1 by shRNA results in defective osteogenic differentiation via cAMP/PKA pathway in human MG-63 cells.

机构信息

Institute of Clinical Pharmacology, Central South University, Changsha, Hunan, 410078, China.

出版信息

J Cell Biochem. 2012 Mar;113(3):967-76. doi: 10.1002/jcb.23426.

Abstract

Mutations and/or deletions of Pkd1 in mouse models resulted in attenuation of osteoblast function and defective bone formation; however, the function of PKD1 in human osteoblast and bone remains uncertain. In the current study, we used lentivirus-mediated shRNA technology to stably knock down PKD1 in the human osteoblastic MG-63 cell line and to investigate the role of PKD1 on human osteoblast function and molecular mechanisms. We found that a 53% reduction of PKD1 by PKD1 shRNA in stable, transfected MG-63 cells resulted in increased cell proliferation and impaired osteoblastic differentiation as reflected by increased BrdU incorporation, decreased alkaline phosphatase activity, and calcium deposition and by decreased expression of RUNX2 and OSTERIX compared to control shRNA MG-63 cells. In addition, knockdown of PKD1 mRNA caused enhanced adipogenesis in stable PKD1 shRNA MG-63 cells as evidenced by elevated lipid accumulation and increased expression of adipocyte-related markers such as PPARγ and aP2. The stable PKD1 shRNA MG-63 cells exhibited lower basal intracellular calcium, which led to attenuated cytosolic calcium signaling in response to fluid flow shear stress, as well as increased intracellular cAMP messages in response to forskolin (10 µM) stimulation. Moreover, increased cell proliferation, inhibited osteoblastic differentiation, and osteogenic and adipogenic gene markers were significantly reversed in stable PKD1 shRNA MG-63 cells when treated with H89 (1 µM), an inhibitor of PKA. These findings suggest that downregulation of PKD1 in human MG-63 cells resulted in defective osteoblast function via intracellular calcium-cAMP/PKA signaling pathway.

摘要

在小鼠模型中,PKd1 的突变和/或缺失导致成骨细胞功能减弱和骨形成缺陷;然而,PKD1 在人类成骨细胞和骨骼中的功能仍然不确定。在本研究中,我们使用慢病毒介导的 shRNA 技术在人成骨细胞 MG-63 细胞系中稳定敲低 PKD1,并研究 PKD1 对人成骨细胞功能的作用及其分子机制。我们发现,稳定转染的 MG-63 细胞中 PKD1 shRNA 使 PKD1 减少 53%,导致细胞增殖增加,成骨分化受损,表现为 BrdU 掺入增加、碱性磷酸酶活性降低、钙沉积减少,以及 RUNX2 和 OSTERIX 的表达降低,与对照 shRNA MG-63 细胞相比。此外,PKD1 mRNA 的敲低导致稳定 PKD1 shRNA MG-63 细胞中的脂肪生成增强,表现为脂滴积累增加和脂肪细胞相关标志物如 PPARγ 和 aP2 的表达增加。稳定的 PKD1 shRNA MG-63 细胞表现出较低的基础细胞内钙,导致对流体剪切力的细胞质钙信号转导减弱,以及对 forskolin(10 µM)刺激的细胞内 cAMP 信号增加。此外,当用 H89(1 µM)处理时,稳定的 PKD1 shRNA MG-63 细胞中的细胞增殖增加、成骨分化抑制、成骨和脂肪生成基因标志物显著逆转,H89 是 PKA 的抑制剂。这些发现表明,PKD1 在人 MG-63 细胞中的下调通过细胞内钙-cAMP/PKA 信号通路导致成骨细胞功能缺陷。

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