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作 者:曹婧[1] 张烨 彭志刚[1] 李际仙[1] 王少鹏[1]
机构地区:[1]中国科学院北京基因组研究所 [2]上海华大天源生物科技有限公司,上海201203
出 处:《中国生物工程杂志》2008年第9期61-67,共7页China Biotechnology
基 金:国家自然科学基金资助项目(30572335)
摘 要:目的:建立基于报告基因的组胺H3受体(H3R)激活剂的高通量筛选模型,用此模型对收集到的中草药化合物组分进行筛选,以发现新的组胺H3R激活剂。方法将H3R基因质粒(H3R/pCDNA3.1-hygro)与报告基因质粒(3XCRE-LUC)按3∶1的比例共转染入HEK293细胞,建立了稳定的H3R配体的报告基因筛选细胞株。激活剂与细胞表面H3R结合后,激活相应的信号通路,调节Forskolin刺激后的报告基因的表达,通过测定荧光素酶报告基因表达水平的变化,评估激活剂影响H3受体的生物活性。结果通过对筛选条件,如激活剂孵育时间、Forskolin终浓度、化合物溶剂的选择、溶剂DMSO终浓度等的优化,建立了可靠的筛选方法。该模型的Z因子可达到0.5以上,稳定性可保持20代,完全符合高通量筛选需求。利用该细胞模型对多种中草药萃取物进行了筛选,找到了两种对H3R有活性的中药组分。结论建立的细胞模型可以有效的应用于以组胺H3受体为靶点的高通量药物筛选。Objective: A cell based reporter gene assay had been established and optimized for high throughput screening to find agonists for human histamine 3 receptor (H3R) from Chinese herb components. Methods : The H3 receptor plasmid (H3R/pCDNA3.1-hygro) and reporter gene plasmid (3XCRE-LUC) were cotransfected HEK293 and a stable cell line was selected with antibiotics for H3 receptor agonist screening. Upon agonist binding, H3 receptor was activated and lead to a decrease of the high expression of luciferase gene induced by forskolin. Result: To identify and optimize the assay condition, the effects of some factors were examined, such as compound solvent selection, final concentration of forskolin, agonist and forskolin incubation time, final concentration of DMSO. A steady cell line and a reliable method were established for H3R agonist screening, the Z'factor value was above 0.5, the signal did not change using HEK/H3R/CRE cell line passage 5 to passage 20. By using this assay system, two herb components were identified and regarded to contain agonists for H3 receptor. Conclusion:This drug screening cell model has been successfully used for histamine 3 receptor target high throughput drug screening.
关 键 词:组胺H3受体(H3R) 报告基因 FORSKOLIN 高通量筛选
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