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首页> 外文期刊>International Journal of Health, Animal Science and Food Safety >Effects of Ghrelin on metabolic activity of equine cartilage affected with inflammatory degeneration: preliminary isolation, characterization of equine cultured chondrocytes and assessment of LPS-induced inflammatory stress.
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Effects of Ghrelin on metabolic activity of equine cartilage affected with inflammatory degeneration: preliminary isolation, characterization of equine cultured chondrocytes and assessment of LPS-induced inflammatory stress.

机译:Ghrelin对受炎性变性影响的马软骨代谢活性的影响:初步分离,马培养的软骨细胞的表征和LPS诱导的炎性应激评估。

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摘要

Ghrelin, the natural ligand for GH secretagogue receptors, influences the activity of both human and rat joint chondrocytes, modulating the synthesis of eicosanoids in the cartilage 1 . This project aims to assess the possible protective effects of Ghrelin on equine cultured chondrocytes exposed to lipopolysaccharide (LPS), as a model of osteoarthritic joint. In the preliminary step of our study, we have characterized equine chondrocyte primary cell cultures and standardized the detrimental effects LPS on chondrocytes health. Equine articular cartilage was collected with aseptic procedure and equine chondrocytes were isolated by overnight incubation. Cells were cultured in monolayer culture to obtain third-passage (P3) chondrocytes and specific cartilaginous genes were identified by qualitative PCR. P3 chondrocytes were treated with increasing LPS concentrations (1-100 ng/ml) and the effects of LPS were assessed with the apoptosis-induction test and fluorescence microscopy after 1, 3, 6, 12, 24, 48 h of treatment. PCR evidenced type II collagenases and aggrecan expression in isolated cells confirming the isolation of chondrocytes. Healthy chondrocytes (HC) showed no fluorescence, necrotic chondrocytes (NC) red fluorescence, early apoptotic chondrocytes (EAC) green fluorescence and advanced apoptotic chondrocytes (AAC) mixed green-red fluorescence. In LPS-stimulated chondrocytes, there was a trend throughout an increased percentage of AAC that became equal to or overwhelmed the percentage of HC after 3 hours for all LPS treatments and lasted for 6 hours after the highest LPS concentration used. On the basis of these results, the concentration of LPS 100 ng/ml for 6 h will be used for subsequent experiments.
机译:Ghrelin,GH促分泌素受体的天然配体,影响人和大鼠关节软骨细胞的活性,调节软骨中类花生酸的合成1。该项目旨在评估Ghrelin对暴露于脂多糖(LPS)的马培养软骨细胞(作为骨关节炎关节的模型)的可能的保护作用。在我们研究的初步步骤中,我们已经对马软骨细胞原代细胞培养进行了表征,并标准化了LPS对软骨细胞健康的有害影响。用无菌方法收集马关节软骨,并通过过夜孵育分离马软骨细胞。在单层培养物中培养细胞以获得第三代(P3)软骨细胞,并通过定性PCR鉴定特定的软骨基因。用增加的LPS浓度(1-100 ng / ml)处理P3软骨细胞,并在处理1、3、6、12、24、48小时后通过凋亡诱导试验和荧光显微镜术评估LPS的作用。 PCR证明II型胶原酶和聚集蛋白聚糖在分离的细胞中表达,证实了软骨细胞的分离。健康的软骨细胞(HC)无荧光,坏死的软骨细胞(NC)红色荧光,早期的凋亡软骨细胞(EAC)绿色荧光和晚期的凋亡软骨细胞(AAC)混合的绿红色荧光。在LPS刺激的软骨细胞中,所有APS处理3小时后,AAC百分比均呈上升趋势,等于或超过HC百分比,并在使用最高LPS浓度后持续6小时。基于这些结果,LPS 100 ng / ml的浓度持续6 h将用于后续实验。

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