使用病毒样颗粒和无标记结合试验生成热稳定的激动剂结合GPR40/FFAR1。

Q3 Biochemistry, Genetics and Molecular Biology Molecular Membrane Biology Pub Date : 2014-08-01 DOI:10.3109/09687688.2014.923588
Yoshihiko Hirozane, Takashi Motoyaji, Takamitsu Maru, Kengo Okada, Naoki Tarui
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引用次数: 12

摘要

阐明膜蛋白受体激活及其配体结合的详细机制对基于结构的药物设计至关重要。膜蛋白晶体结构分析成功地帮助理解这些基本的分子相互作用。然而,g蛋白偶联受体(GPCR)的蛋白质晶体结构分析仍然具有挑战性,即使对于大多数膜蛋白结构分析报告中包含的GPCR类,由于这些受体在从脂质双层膜中提取时具有很大的不稳定性。众所周知,热稳定性的增加往往会降低构象柔韧性,这有助于生成衍射质量的晶体。然而,这仍然不是直截了当的,并且需要大量的努力来确定最适合晶体学的热稳定突变体。为了解决这一问题,开发了一种基于无标记配体结合试验结合病毒样颗粒瞬时过表达的多功能筛选平台。该平台用于生成法西lifam (TAK-875)的热稳定GPR40[也称为游离脂肪酸受体1 (FFAR1)]。这表明热稳定突变体GPR40 (L42A/F88A/G103A/Y202F)可以成功用于晶体结构分析。
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Generating thermostabilized agonist-bound GPR40/FFAR1 using virus-like particles and a label-free binding assay.

Elucidating the detailed mechanism of activation of membrane protein receptors and their ligand binding is essential for structure-based drug design. Membrane protein crystal structure analysis successfully aids in understanding these fundamental molecular interactions. However, protein crystal structure analysis of the G-protein-coupled receptor (GPCR) remains challenging, even for the class of GPCRs which have been included in the majority of structure analysis reports among membrane proteins, due to the substantial instability of these receptors when extracted from lipid bilayer membranes. It is known that increased thermostability tends to decrease conformational flexibility, which contributes to the generation of diffraction quality crystals. However, this is still not straightforward, and significant effort is required to identify thermostabilized mutants that are optimal for crystallography. To address this issue, a versatile screening platform based on a label-free ligand binding assay combined with transient overexpression in virus-like particles was developed. This platform was used to generate thermostabilized GPR40 [also known as free fatty acid receptor 1 (FFAR1)] for fasiglifam (TAK-875). This demonstrated that the thermostabilized mutant GPR40 (L42A/F88A/G103A/Y202F) was successfully used for crystal structure analysis.

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来源期刊
Molecular Membrane Biology
Molecular Membrane Biology 生物-生化与分子生物学
CiteScore
4.80
自引率
0.00%
发文量
0
审稿时长
>12 weeks
期刊介绍: Cessation. Molecular Membrane Biology provides a forum for high quality research that serves to advance knowledge in molecular aspects of biological membrane structure and function. The journal welcomes submissions of original research papers and reviews in the following areas: • Membrane receptors and signalling • Membrane transporters, pores and channels • Synthesis and structure of membrane proteins • Membrane translocation and targeting • Lipid organisation and asymmetry • Model membranes • Membrane trafficking • Cytoskeletal and extracellular membrane interactions • Cell adhesion and intercellular interactions • Molecular dynamics and molecular modelling of membranes. • Antimicrobial peptides.
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