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琼脂糖培养中软骨细胞簇形成作为一种功能测定法,用于鉴定骨关节炎中表达的基因。

Chondrocyte cluster formation in agarose cultures as a functional assay to identify genes expressed in osteoarthritis.

作者信息

Quintavalla Joseph, Kumar Chandrika, Daouti Sherif, Slosberg Eric, Uziel-Fusi Susan

机构信息

Department of Bone, Muscle and Gastrointestinal, Novartis Institutes for BioMedical Research, East Hanover, New Jersey, USA.

出版信息

J Cell Physiol. 2005 Aug;204(2):560-6. doi: 10.1002/jcp.20345.

DOI:10.1002/jcp.20345
PMID:15799031
Abstract

Understanding altered gene expression in osteoarthritic cartilage can lead to new targets for drug intervention. We established a functional assay based on chondrocyte cluster formation, a phenotype associated with osteoarthritis (OA), to screen an OA cartilage gene library. Previous reports have demonstrated that normal chondrocytes grown in suspension culture maintain their chondrocytic phenotype, however, certain growth factors such as basic fibroblast growth factor (bFGF) will induce the cells to proliferate in tight clusters similar to those seen in osteoarthritic cartilage. In this study we validate that overexpression of bFGF by retrovirally transduced normal chondrocytes would similarly induce the proliferation of tight cell clusters. We then used this approach as a basis to set up a functional screen where an entire OA cartilage cDNA library was tranduced into normal chondrocytes to search for other genes that would also induce cluster formation. Seven potential genes were isolated from the OA gene library, including BPOZ, IL-17 receptor C, NADH ubiquinone oxidoreductase, COMP, Soluble carrier 16 (MCT 3), C1r, and bFGF itself. None of the identified genes were upregulated by bFGF, however, all of them upregulated the expression of bFGF suggesting a common pathway. Although cluster formation is not considered to be destructive in OA cartilage, it is consistent with the disease and could yield answers to the altered phenotype. Further studies are needed to elucidate how these genes are linked to the disease state.

摘要

了解骨关节炎软骨中基因表达的改变可为药物干预提供新靶点。我们基于软骨细胞簇形成(一种与骨关节炎(OA)相关的表型)建立了一种功能检测方法,以筛选OA软骨基因文库。先前的报道表明,悬浮培养的正常软骨细胞可维持其软骨细胞表型,然而,某些生长因子,如碱性成纤维细胞生长因子(bFGF),会诱导细胞紧密聚集增殖,类似于在骨关节炎软骨中所见。在本研究中,我们验证了通过逆转录病毒转导正常软骨细胞使bFGF过表达同样会诱导紧密细胞簇的增殖。然后,我们以此方法为基础建立了一个功能筛选,将整个OA软骨cDNA文库转导至正常软骨细胞中,以寻找其他也能诱导簇形成的基因。从OA基因文库中分离出7个潜在基因,包括BPOZ、IL-17受体C、NADH泛醌氧化还原酶、COMP、可溶性载体16(MCT 3)、C1r和bFGF自身。所鉴定的基因均未被bFGF上调,然而,它们均上调了bFGF的表达,提示存在一条共同途径。尽管簇形成在OA软骨中不被认为具有破坏性,但它与该疾病相符,并且可能为表型改变提供答案。需要进一步研究来阐明这些基因如何与疾病状态相关联。

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