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成骨细胞与成软骨细胞分化

Osteoblast and chondroblast differentiation.

作者信息

Aubin J E, Liu F, Malaval L, Gupta A K

机构信息

Department of Anatomy and Cell Biology, University of Toronto, Ontario, Canada.

出版信息

Bone. 1995 Aug;17(2 Suppl):77S-83S. doi: 10.1016/8756-3282(95)00183-e.

DOI:10.1016/8756-3282(95)00183-e
PMID:8579903
Abstract

Recognition of discrete commitment and differentiation stages requires characterization of changes in proliferative capacity together with the temporal acquisition or loss of expression of molecular and morphological traits. Both cell lines and primary cultures have been useful for analysis of transitional steps in the chondroblast (CB) and osteoblast (OB) lineages. One striking feature is that OBs and CBs share expression of some molecules, including newer markers such as epsilon BP (galectin-3), while also having unique markers. The fact that hypertrophic chondrocytes appear able to downregulate cartilage markers and upregulate OB markers also points to an interesting lineage relationship that needs to be explored further. Recently, we have focused on the osteoprogenitors that divide and differentiate into mature OBs forming bone nodules in fetal rat calvaria cell cultures. We use cellular, immunocytochemical, and molecular approaches, including PCR on small numbers of cells, to discriminate stages. Nodule formation is characterized by loss of proliferative capacity and sequential increased marker expression, that is, alkaline phosphatase (AP), followed by bone sialoprotein (BSP), and osteocalcin. Upregulation of collagen type I and biphasic expression of osteopontin, with two peaks corresponding to proliferation and differentiation stages, also occurs. A variety of other molecules are also upregulated in the mature OB, including epsilon BP and CD44s. By replica plating and PCR, we have begun to study the expression of the messenger RNAs (mRNAs) for potential regulatory molecules (e.g., PTHrP) and their receptors (e.g., PTHR, FGFR-1, and PDGFR alpha) and have found all to be modulated during the progression from committed osteoprogenitor to mature OB.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

识别离散的定向分化阶段需要对增殖能力的变化以及分子和形态特征表达的暂时获得或丧失进行表征。细胞系和原代培养物对于分析成软骨细胞(CB)和成骨细胞(OB)谱系中的过渡步骤都很有用。一个显著特征是,成骨细胞和成软骨细胞共享一些分子的表达,包括一些新的标志物,如εBP(半乳糖凝集素-3),同时也有独特的标志物。肥大软骨细胞似乎能够下调软骨标志物并上调成骨细胞标志物,这一事实也表明了一种有趣的谱系关系,需要进一步探索。最近,我们专注于在胎鼠颅骨细胞培养物中分裂并分化为形成骨结节的成熟成骨细胞的骨祖细胞。我们使用细胞、免疫细胞化学和分子方法,包括对少量细胞进行PCR,来区分不同阶段。结节形成的特征是增殖能力丧失和标志物表达顺序增加,即碱性磷酸酶(AP),随后是骨唾液蛋白(BSP)和骨钙素。I型胶原蛋白上调以及骨桥蛋白的双相表达,两个峰值分别对应增殖和分化阶段,也会发生。成熟成骨细胞中还上调了多种其他分子,包括εBP和CD44s。通过复制铺板和PCR,我们已经开始研究潜在调节分子(如甲状旁腺激素相关蛋白(PTHrP))及其受体(如甲状旁腺激素受体(PTHR)、成纤维细胞生长因子受体-1(FGFR-1)和血小板衍生生长因子受体α(PDGFRα))的信使核糖核酸(mRNA)表达,并且发现所有这些在从定向骨祖细胞到成熟成骨细胞的进程中都会受到调节。(摘要截短至250字)

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