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体外对一种骨骼细胞系(CFK2)中软骨细胞表型表达的调控。

Regulation of expression of the chondrocytic phenotype in a skeletal cell line (CFK2) in vitro.

作者信息

Bernier S M, Goltzman D

机构信息

Calcium Research Laboratory, McGill University, Montréal, Québec, Canada.

出版信息

J Bone Miner Res. 1993 Apr;8(4):475-84. doi: 10.1002/jbmr.5650080412.

DOI:10.1002/jbmr.5650080412
PMID:8475797
Abstract

We have examined in vitro the spontaneous and regulated expression of phenotypic characteristics associated with differentiated chondrocytes in an established skeletal cell line (CFK2) derived from fetal rat calvariae. Extended culture of CFK2 cells resulted in the appearance of glycosaminoglycans and type II collagen in the cell layer in association with the formation of focal nodes of cells. In addition, induction of mRNA-encoding link protein, cartilage-specific proteoglycan core protein, and thrombospondin was observed in the differentiated population (dCFK2 cells). The expression of these mRNAs was present for at least two passages after subculturing the dCFK2 cells. The dCFK2 cells also demonstrated enhanced parathyroid hormone (PTH)-stimulated adenylate cyclase activity. Proliferation of CFK2 cells was stimulated by the peptide regulatory factors EGF and PTH and inhibited by the steroidal agents dexamethasone and retinoic acid. EGF and retinoic acid inhibited the formation of cell foci and glycosaminoglycan deposition and the expression of mRNA-encoding link protein. In contrast, PTH and dexamethasone enhanced the formation of focal cellular nodes and augmented matrix deposition and link protein mRNA expression. These studies therefore show that the CFK2 cell line can serve as a nontransformed model of rat chondrocytic cells in which both induction and regulation of the expression of cartilaginous matrix components can be observed. This line thereby provides a unique renewable source of chondrocytic precursor cells and an excellent in vitro model for evaluating temporal and environmental control of chondrocyte differentiation and cartilage matrix production.

摘要

我们已经在体外研究了源自胎鼠颅骨的成熟骨骼细胞系(CFK2)中与分化软骨细胞相关的表型特征的自发表达和调控表达。CFK2细胞的长期培养导致细胞层中出现糖胺聚糖和II型胶原蛋白,并伴有细胞灶性结节的形成。此外,在分化群体(dCFK2细胞)中观察到编码连接蛋白、软骨特异性蛋白聚糖核心蛋白和血小板反应蛋白的mRNA的诱导。在dCFK2细胞传代培养后,这些mRNA的表达至少持续了两代。dCFK2细胞还表现出甲状旁腺激素(PTH)刺激的腺苷酸环化酶活性增强。CFK2细胞的增殖受到肽调节因子EGF和PTH的刺激,并受到甾体药物地塞米松和视黄酸的抑制。EGF和视黄酸抑制细胞灶的形成、糖胺聚糖沉积以及编码连接蛋白的mRNA的表达。相反,PTH和地塞米松增强了细胞灶性结节的形成,增加了基质沉积和连接蛋白mRNA的表达。因此,这些研究表明CFK2细胞系可作为大鼠软骨细胞的非转化模型,在其中可以观察到软骨基质成分表达的诱导和调控。该细胞系从而提供了一种独特的可再生软骨细胞前体细胞来源,以及一个用于评估软骨细胞分化和软骨基质产生的时间和环境控制的优秀体外模型。

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