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利用新型酵母/哺乳动物G蛋白α亚基嵌合体实现哺乳动物受体与酵母交配途径的功能偶联。

Functional coupling of mammalian receptors to the yeast mating pathway using novel yeast/mammalian G protein alpha-subunit chimeras.

作者信息

Brown A J, Dyos S L, Whiteway M S, White J H, Watson M A, Marzioch M, Clare J J, Cousens D J, Paddon C, Plumpton C, Romanos M A, Dowell S J

机构信息

Molecular Pharmacology Unit, Glaxo Wellcome Medicines Research Centre, Gunnels Wood Road, Stevenage, Hertfordshire SG1 2NY, UK.

出版信息

Yeast. 2000 Jan 15;16(1):11-22. doi: 10.1002/(SICI)1097-0061(20000115)16:1<11::AID-YEA502>3.0.CO;2-K.

DOI:10.1002/(SICI)1097-0061(20000115)16:1<11::AID-YEA502>3.0.CO;2-K
PMID:10620771
Abstract

The expression of mammalian G protein coupled receptors (GPCRs) in S. cerevisiae provides a powerful assay system for functional analysis, ligand identification and pharmaceutical screening. However, relatively few receptors have been coupled to the pheromone response pathway via the yeast G(alpha), Gpa1p, or chimeric yeast/mammalian G(alpha) subunits containing long C-terminal regions of mammalian G(alpha) proteins. We tested an extended range of seven such chimeras for G(alpha) sub-types of three major classes (G(alphai/o), G(alphas) and G(alphaq)), against eight human GPCRs (SST(2), SST(5), 5-HT(1A), 5-HT(1Dalpha), ML(1B), P2Y(1) and P2Y(2)). Although the G(alphai/o) chimeras increased the range of receptors that coupled efficiently, the G(alphas) and G(alphaq) chimeras were inactive when expressed using the GPA1 promoter. We describe 10 novel Gpa1p chimeras, designated 'transplants', in which the C-terminal five amino acids of Gpa1p were exchanged with mammalian residues. Coupling efficiency and ligand sensitivity improved significantly using the transplants. For the P2Y purinergic receptors, coupling could only be detected with the transplants; this is the first report of G(q) specificity coupling in yeast. Thus, the transplants offer major advantages over previously described approaches, in terms of both the range of receptors coupled and the efficiency of coupling.

摘要

哺乳动物G蛋白偶联受体(GPCRs)在酿酒酵母中的表达为功能分析、配体鉴定和药物筛选提供了一个强大的检测系统。然而,相对较少的受体通过酵母Gα亚基Gpa1p或包含哺乳动物Gα蛋白长C端区域的酵母/哺乳动物嵌合Gα亚基与信息素反应途径偶联。我们针对三种主要类型(Gαi/o、Gαs和Gαq)的Gα亚型,测试了七种此类嵌合体与八种人类GPCR(SST2、SST5、5-HT1A、5-HT1Dα、ML1B、P2Y1和P2Y2)的广泛组合。尽管Gαi/o嵌合体增加了有效偶联受体的范围,但使用GPA1启动子表达时,Gαs和Gαq嵌合体无活性。我们描述了10种新型的Gpa1p嵌合体,命名为“移植体”,其中Gpa1p的C端五个氨基酸被哺乳动物残基取代。使用这些移植体时,偶联效率和配体敏感性显著提高。对于P2Y嘌呤能受体,只有使用移植体才能检测到偶联;这是酵母中Gq特异性偶联的首次报道。因此,就偶联受体的范围和偶联效率而言,移植体比先前描述的方法具有主要优势。

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