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通过细菌发酵制备稳定同位素标记的外周大麻素受体CB2

Preparation of stable isotope-labeled peripheral cannabinoid receptor CB2 by bacterial fermentation.

作者信息

Berger Christian, Ho Jenny T C, Kimura Tomohiro, Hess Sonja, Gawrisch Klaus, Yeliseev Alexei

机构信息

Institute for Biochemistry and Biotechnology, Martin-Luther University, Halle-Wittenberg, Kurt-Mothes-Str., 3, 06120 Halle, Germany.

出版信息

Protein Expr Purif. 2010 Apr;70(2):236-47. doi: 10.1016/j.pep.2009.12.011. Epub 2010 Jan 4.

DOI:10.1016/j.pep.2009.12.011
PMID:20044006
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2827653/
Abstract

We developed a bacterial fermentation protocol for production of a stable isotope-labeled cannabinoid receptor CB2 for subsequent structural studies of this protein by nuclear magnetic resonance spectroscopy. The human peripheral cannabinoid receptor was expressed in Escherichia coli as a fusion with maltose binding protein and two affinity tags. The fermentation was performed in defined media comprised of mineral salts, glucose and (15)N(2)-L-tryptophan to afford incorporation of the labeled amino acid into the protein. Medium, growth and expression conditions were optimized so that the fermentation process produced about 2mg of purified, labeled CB2/L of culture medium. By performing a mass spectroscopic characterization of the purified CB2, we determined that one of the two (15)N atoms in tryptophan was incorporated into the recombinant protein. NMR analysis of (15)N chemical shifts strongly suggests that the (15)N atoms are located in Trp-indole rings. Importantly, analysis of the peptides derived from the CNBr cleavage of the purified protein confirmed a minimum of 95% incorporation of the labeled tryptophan into the CB2 sequence. The labeled CB2, purified and reconstituted into liposomes at a protein-to-lipid molar ratio of 1:500, was functional as confirmed by activation of cognate G proteins in an in vitro coupled assay. To our knowledge, this is the first reported production of a biologically active, stable isotope-labeled G protein-coupled receptor by bacterial fermentation.

摘要

我们开发了一种细菌发酵方案,用于生产稳定同位素标记的大麻素受体CB2,以便随后通过核磁共振光谱对该蛋白质进行结构研究。人外周大麻素受体在大肠杆菌中作为与麦芽糖结合蛋白和两个亲和标签的融合蛋白表达。发酵在由矿物盐、葡萄糖和(15)N(2)-L-色氨酸组成的限定培养基中进行,以使标记的氨基酸掺入蛋白质中。对培养基、生长和表达条件进行了优化,从而使发酵过程每升培养基产生约2mg纯化的、标记的CB2。通过对纯化的CB2进行质谱表征,我们确定色氨酸中的两个(15)N原子之一被掺入重组蛋白中。对(15)N化学位移的NMR分析强烈表明(15)N原子位于色氨酸吲哚环中。重要的是,对纯化蛋白经溴化氰裂解得到的肽段的分析证实,标记的色氨酸至少有95%掺入CB2序列中。纯化后的标记CB2以1:500的蛋白质与脂质摩尔比重构到脂质体中,在体外偶联试验中通过同源G蛋白的激活证实其具有功能。据我们所知,这是首次报道通过细菌发酵生产具有生物活性的、稳定同位素标记的G蛋白偶联受体。

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