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Inhibition of lysyl oxidase activity can delay phenotypic modulation of chondrocytes in two-dimensional culture.

机译:赖氨酰氧化酶活性的抑制可延迟二维培养中软骨细胞的表型调节。

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OBJECTIVE: Chondrocytes frequently de-differentiate in two-dimensional (2D) culture, especially in the presence of serum. To examine the role of lysyl oxidase (LOX) induced cross-linking in this phenomenon, the effect of the specific LOX inhibitor beta-aminopropionitrile (BAPN) was studied in 2D chondrocyte culture. DESIGN: Chick embryo sternal chondrocytes (both proliferative and hypertrophic, from caudal and cranial zones, respectively) were cultured in the presence and absence of BAPN. The production and activities of LOX and LOX-like (LOXL) were assessed by enzyme assay and the use of specific antibodies. Seventeen batches of serum of different origin were compared. Chondrocyte phenotype was assessed both morphologically and biochemically, the latter by quantitative analysis of production of radiolabeled cartilage collagens II, IX, X and XI, and the de-differentiation marker collagen I, for up to 4 weeks in culture. RESULTS: LOX and LOXL were identified, by Western blotting and immunofluorescence, and LO activity was measured in the medium, with both proliferative and hypertrophic chondrocytes. Inhibition of LO activity prevented or delayed chondrocyte de-differentiation, as characterized by changes in cell shape and synthesis of the five different collagen types, from the first days of culture for up to 4 weeks, depending on the origin of the serum added to the culture medium. CONCLUSION: LO activity may be involved in the control of chondrocyte phenotype, in addition to serum factors. Inhibition of LO activity by BAPN may be useful for the maintenance of the chondrocyte phenotype in 2D culture. Specific variations in the relative proportions of collagens II, IX and XI could be involved in the mechanism underlying these observations.
机译:目的:软骨细胞在二维(2D)培养中经常去分化,尤其是在存在血清的情况下。若要检查赖氨酰氧化酶(LOX)诱导的交联在此现象中的作用,在二维软骨细胞培养物中研究了特定LOX抑制剂β-氨基丙腈(BAPN)的作用。设计:在有和没有BAPN的情况下培养小鸡的胚胎胸骨软骨细胞(分别来自尾和颅区的增生和肥大细胞)。通过酶测定和特异性抗体的使用来评估LOX和LOX样(LOXL)的产生和活性。比较了十七批不同来源的血清。在形态学和生化方面评估软骨细胞的表型,后者通过对放射性标记的胶原蛋白II,IX,X和XI以及去分化标记物胶原蛋白I的产生进行定量分析,在培养中长达4周。结果:通过Western印迹和免疫荧光鉴定了LOX和LOXL,并在培养基中测量了增殖和肥大软骨细胞的LO活性。抑制LO活性可防止或延迟软骨细胞去分化,其特征是从培养的第一天开始长达4周,这取决于细胞形状的变化和五种不同胶原蛋白类型的合成,具体取决于添加到血清中的血清来源。培养基。结论:除血清因素外,LO活性可能还参与了软骨细胞表型的控制。 BAPN对LO活性的抑制可能对维持2D培养中的软骨细胞表型有用。这些观察结果的基础机制可能涉及胶原II,IX和XI相对比例的特定变化。

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