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凝集素结合模式反映了体外软骨细胞模型的表型状态。

Lectin binding patterns reflect the phenotypic status of in vitro chondrocyte models.

作者信息

Toegel S, Plattner V E, Wu S Q, Goldring M B, Chiari C, Kolb A, Unger F M, Nehrer S, Gabor F, Viernstein H, Wirth M

机构信息

Medical University Vienna, Waehringer Guertel 18-20, 1090 Vienna, Austria.

出版信息

In Vitro Cell Dev Biol Anim. 2009 Jul-Aug;45(7):351-60. doi: 10.1007/s11626-009-9186-5. Epub 2009 Mar 5.

Abstract

In vitro studies using chondrocyte cell cultures have increased our understanding of cartilage physiology and the altered chondrocytic cell phenotype in joint diseases. Beside the use of primary cells isolated from cartilage specimens of donors, immortalized chondrocyte cell lines such as C-28/I2 and T/C-28a2 have facilitated reproducible and standardized experiments. Although carbohydrate structures appear of significance for cartilage function, the contribution of the chondrocyte glycocalyx to matrix assembly and alterations of the chondrocyte phenotype is poorly understood. Therefore, the present study aimed to evaluate the glycoprofile of primary human chondrocytes as well as of C-28/I2 and T/C-28a2 cells in culture. First, the chondrocytic phenotype of primary and immortalized cells was assessed using real-time reverse transcriptase polymerase chain reaction, immunofluorescence, and glycosaminoglycans staining. Then, a panel of lectins was selected to probe for a range of oligosaccharide sequences determining specific products of the O-glycosylation and N-glycosylation pathways. We found that differences in the molecular phenotype between primary chondrocytes and the immortalized chondrocyte cell models C-28/I2 and T/C-28a2 are reflected in the glycoprofile of the cells. In this regard, the glycocalyx of immortalized chondrocytes was characterized by reduced levels of high-mannose type and sialic acid-capped N-glycans as well as increased fucosylated O-glycosylation products. In summary, the present report emphasizes the glycophenotype as an integral part of the chondrocyte phenotype and points at a significant role of the glycophenotype in chondrocyte differentiation.

摘要

使用软骨细胞培养物进行的体外研究增进了我们对软骨生理学以及关节疾病中软骨细胞表型改变的理解。除了使用从供体软骨标本中分离的原代细胞外,永生化软骨细胞系,如C-28/I2和T/C-28a2,促进了可重复和标准化的实验。尽管碳水化合物结构似乎对软骨功能很重要,但软骨细胞糖萼对基质组装和软骨细胞表型改变的贡献却知之甚少。因此,本研究旨在评估培养的原代人软骨细胞以及C-28/I2和T/C-28a2细胞的糖谱。首先,使用实时逆转录聚合酶链反应、免疫荧光和糖胺聚糖染色评估原代细胞和永生化细胞的软骨细胞表型。然后,选择一组凝集素来探测一系列寡糖序列,这些序列决定了O-糖基化和N-糖基化途径的特定产物。我们发现,原代软骨细胞与永生化软骨细胞模型C-28/I2和T/C-28a2之间的分子表型差异反映在细胞的糖谱中。在这方面,永生化软骨细胞的糖萼特征是高甘露糖型和唾液酸封端的N-聚糖水平降低,以及岩藻糖基化的O-糖基化产物增加。总之,本报告强调糖表型是软骨细胞表型的一个组成部分,并指出糖表型在软骨细胞分化中具有重要作用。

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