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首页> 外文期刊>Journal of Immunological Methods >A novel cell-based system for the rapid quantitative evaluation of (anti)-inflammatory potential of test substances.
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A novel cell-based system for the rapid quantitative evaluation of (anti)-inflammatory potential of test substances.

机译:一种新型的基于细胞的系统,用于快速定量评估测试物质的(抗)炎症潜能。

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摘要

The control of NF-kappaB activation is a proven therapeutic strategy in the treatment of multiple inflammatory disorders. Drug discovery and development for such a therapy demands a battery of assays to reliably demonstrate both clinical effectiveness and biological safety of prospective medications. Unlike traditional in vitro biochemical analyses, cell-based assays more closely mimic the actual in vivo physiologic environment, addressing simultaneously biological activity and toxicity issues. A novel assay system, based solely on the drug resistance of a genetically engineered cell line, has been developed to provide rapid quantitative evaluation of the (anti)-inflammatory potential of test substances. The assay principle is based on the ability of bona fide inflammatory agents to activate the transcription factor NF-kappaB in cultured cells. In our model, expression of a dual drug resistance marker, driven by an NF-kappaB-dependent minimal promoter, provides a selective and highly sensitive scheme with a quantitative readout to detect biochemical agents with pro-or anti-inflammatory properties. The novel cell-based system is inexpensive, simple to perform (requiring only basic cell culture skills), accurate, and provides sensitivity comparable to that of the electrophoretic mobility shift assay and quantitative ELISA. In addition, the dual selection capability of the model provides a powerful tool to discover novel molecular components of the NF-kappaB signal transduction pathway.
机译:在多种炎症性疾病的治疗中,控制NF-κB激活是一种行之有效的治疗策略。用于这种疗法的药物发现和开发需要一系列分析方法,以可靠地证明预期药物的临床有效性和生物安全性。与传统的体外生化分析不同,基于细胞的分析更紧密地模拟了实际的体内生理环境,同时解决了生物活性和毒性问题。已经开发了一种仅基于基因工程细胞系的耐药性的新颖测定系统,以提供对测试物质的(抗)炎症潜能的快速定量评估。该测定原理基于真正的炎症剂激活培养细胞中转录因子NF-κB的能力。在我们的模型中,由NF-κB依赖性最小启动子驱动的双重耐药标记的表达提供了选择性和高度敏感的方案,并具有定量读数以检测具有促炎或抗炎特性的生化试剂。这种新颖的基于细胞的系统价格便宜,操作简单(仅需要基本的细胞培养技能),准确,并提供与电泳迁移率变动分析和定量ELISA相当的灵敏度。此外,该模型的双重选择功能为发现NF-κB信号转导途径的新型分子成分提供了强大的工具。

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