A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist

ZHI-HUI ZHENG; GUO-PING LV; SHU-YI SI; YUE-SHENG DONG; BAO-HUA ZHAO; HUA ZHANG; JIAN-GONG HE

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Volume 20 Issue 6

Dec. 2007

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Article Navigation > Biomedical and Environmental Sciences > 2007 > 20(6): 465-469

ZHI-HUI ZHENG, GUO-PING LV, SHU-YI SI, YUE-SHENG DONG, BAO-HUA ZHAO, HUA ZHANG, JIAN-GONG HE. A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist[J]. Biomedical and Environmental Sciences, 2007, 20(6): 465-469.

Citation:

ZHI-HUI ZHENG, GUO-PING LV, SHU-YI SI, YUE-SHENG DONG, BAO-HUA ZHAO, HUA ZHANG, JIAN-GONG HE. A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist[J]. Biomedical and Environmental Sciences, 2007, 20(6): 465-469.

A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist

Insitute of Medicinal Biotechnology, Peking Union Medical College/Chinese Academy of Medical Sciences, Beijing 100050, China;New Drug Research & Development Center of North China Pharmaceutical Group Corporation, National Microbial Medicine Engineering & Research Center, Shijiazhuang 050015, Hebei, China
College of Life Science, Hebei Normal University, Shijiazhuang 050016, Hebei, China
Insitute of Medicinal Biotechnology, Peking Union Medical College/Chinese Academy of Medical Sciences, Beijing 100050, China
New Drug Research & Development Center of North China Pharmaceutical Group Corporation, National Microbial Medicine Engineering & Research Center, Shijiazhuang 050015, Hebei, China

Funds: 科技部资助项目%PRC in Mega-projects of Science Research During the 10th Five-Year Plan Period(2004AA2Z38784)%国家自然科学基金(30472026)

Abstract

Objective To develop a high-throughput screening assay for Farnesoid X receptor (FXR) agonists based on mammalian one-hybrid system (a chimera receptor gene system) for the purpose of identifying new lead compounds for dyslipidaemia drug from the chemical library. Methods cDNA encoding the human FXR ligand binding domain (LBD) was amplified by RT-PCR from a human liver total mRNA and fused to the DNA binding domain (DBD) of yeast GAL4 of pBIND to construct a GAL4-FXR (LBD) chimera expression plasmid. Five copies of the GAL4 DNA binding site were synthesized and inserted into upstream of the SV40 promoter of pGL3-promoter vector to construct a reporter plasmid pG5-SV40 Luc. The assay was developed by transient co-transfection with pG5-SV40 Luc reporter plasmid and pBIND-FXR-LBD (189-472) chimera expression plasmid. Results After optimization, CDCA, a FXR natural agonist, could induce expression of the luciferase gene in a dose-dependent manner, and had a signal/noise ratio of 10 and Z'factor value of 0.65. Conclusion A stable and sensitive cell-based high-throughput screening model can be used in high-throughput screening for FXR agonists from the synthetic and natural compound library.
- Farnesoid X receptor,
- Agonist,
- High-throughput screening,
- Chimera
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通讯作者: 陈斌, bchen63@163.com

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沈阳化工大学材料科学与工程学院沈阳 110142

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A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist

Insitute of Medicinal Biotechnology, Peking Union Medical College/Chinese Academy of Medical Sciences, Beijing 100050, China;New Drug Research & Development Center of North China Pharmaceutical Group Corporation, National Microbial Medicine Engineering & Research Center, Shijiazhuang 050015, Hebei, China

College of Life Science, Hebei Normal University, Shijiazhuang 050016, Hebei, China

Insitute of Medicinal Biotechnology, Peking Union Medical College/Chinese Academy of Medical Sciences, Beijing 100050, China

New Drug Research & Development Center of North China Pharmaceutical Group Corporation, National Microbial Medicine Engineering & Research Center, Shijiazhuang 050015, Hebei, China

Funds: 科技部资助项目%PRC in Mega-projects of Science Research During the 10th Five-Year Plan Period(2004AA2Z38784)%国家自然科学基金(30472026)

Key words:

Abstract: Objective To develop a high-throughput screening assay for Farnesoid X receptor (FXR) agonists based on mammalian one-hybrid system (a chimera receptor gene system) for the purpose of identifying new lead compounds for dyslipidaemia drug from the chemical library. Methods cDNA encoding the human FXR ligand binding domain (LBD) was amplified by RT-PCR from a human liver total mRNA and fused to the DNA binding domain (DBD) of yeast GAL4 of pBIND to construct a GAL4-FXR (LBD) chimera expression plasmid. Five copies of the GAL4 DNA binding site were synthesized and inserted into upstream of the SV40 promoter of pGL3-promoter vector to construct a reporter plasmid pG5-SV40 Luc. The assay was developed by transient co-transfection with pG5-SV40 Luc reporter plasmid and pBIND-FXR-LBD (189-472) chimera expression plasmid. Results After optimization, CDCA, a FXR natural agonist, could induce expression of the luciferase gene in a dose-dependent manner, and had a signal/noise ratio of 10 and Z'factor value of 0.65. Conclusion A stable and sensitive cell-based high-throughput screening model can be used in high-throughput screening for FXR agonists from the synthetic and natural compound library.

Citation:

ZHI-HUI ZHENG, GUO-PING LV, SHU-YI SI, YUE-SHENG DONG, BAO-HUA ZHAO, HUA ZHANG, JIAN-GONG HE. A Cell-based High-throughput Screening Assay for Farnesoid X Recepter Agonist[J]. Biomedical and Environmental Sciences, 2007, 20(6): 465-469.