首页> 外文期刊>Journal of Asian natural products research >Development of a cell-based high-throughput peroxisome proliferator- activated receptors (PPARs) screening model and its application for evaluation of the extracts from Rhizoma Coptis
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Development of a cell-based high-throughput peroxisome proliferator- activated receptors (PPARs) screening model and its application for evaluation of the extracts from Rhizoma Coptis

机译:基于细胞的高通量过氧化物酶体增殖物激活受体(PPARs)筛选模型的开发及其在评估黄连提取物中的应用

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To date, peroxisome proliferator-activated receptors (PPARs) are becoming the new therapeutic targets for the treatment of metabolic diseases, such as Type 2 diabetes, obesity, and cardiovascular disease. In this study, a cell-based high-throughput PPARs (PPAR/β/γ) model was developed for the screening of PPARs agonists. The screening conditions were evaluated through analyzing the expression value of luciferase. Finally, 24 h of drug acting time, 5 times of the dilution factor of luciferase zymolyte, and about 2 × 104 cells/well on HeLa cells in 96-well plates were used, respectively. Furthermore, the quality of high-throughput screening (HTS) in stability and reliability was evaluated by the Z′-factor. Additionally, different extracts of Rhizoma Coptis and berberine were tested by the developed method. The results suggested that both the EtOAc extract and berberine were able to activate PPAR/β/γ, and Rhizoma Coptis contains potential natural agonists of PPARs besides berberine. In conclusion, the developed HTS assay is a simple, rapid, stable, and specific method for the screening of PPARs natural agonists.
机译:迄今为止,过氧化物酶体增殖物激活受体(PPAR)已成为治疗代谢性疾病(如2型糖尿病,肥胖症和心血管疾病)的新治疗靶标。在这项研究中,开发了基于细胞的高通量PPAR(PPAR /β/γ)模型,用于筛选PPAR激动剂。通过分析荧光素酶的表达值来评估筛选条件。最后,在96孔板中分别使用24小时的药物作用时间,5倍的荧光素酶合酶稀释因子和HeLa细胞上的约2×104细胞/孔。此外,通过Z'因子评估了高通量筛选(HTS)在稳定性和可靠性方面的质量。此外,通过开发的方法测试了黄连和小ber碱的不同提取物。结果表明,EtOAc提取物和小ber碱均能够激活PPAR /β/γ,而黄连除小ber碱外还含有潜在的PPARs天然激动剂。总之,开发的HTS分析是一种简单,快速,稳定且特定的PPARs天然激动剂筛选方法。

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