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Nanodisc-based Co-immunoprecipitation for Mass Spectrometric Identification of Membrane-interacting Proteins

机译:基于纳米光盘的免疫共沉淀质谱法鉴定膜相互作用蛋白

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摘要

Proteomic identification of protein interactions with membrane associated molecules in their native membrane environment pose a challenge because of technical problems of membrane handling. We investigate the possibility of employing membrane nanodiscs for harboring the membrane associated molecule to tackle the challenges. Nanodiscs are stable, homogenous pieces of membrane with a discoidal shape. They are stabilized by an encircling amphipatic protein with an engineered epitope tag. In the present study we employ the epitope tag of the nanodiscs for detection and co-immunoprecipitation of interaction partners of the glycolipid ganglioside GM1 harbored by nanodiscs. Highly specific binding activity for nanodisc-GM1 immobilized on sensorchips was observed by surface plasmon resonance in culture media from enterotoxigenic Escherischia coli. To isolate the interaction partner(s) from enterotoxigenic Escherischia coli, GM1-nanodiscs were employed for co-immunoprecipitation. The B subunit of heat labile enterotoxin was identified as a specific interaction partner by mass spectrometry, thus demonstrating that nanodisc technology is useful for highly specific detection and identification of interaction partners to specific lipids embedded in a membrane bilayer.
机译:由于膜处理的技术问题,蛋白质组学鉴定蛋白质与膜相关分子在其天然膜环境中的相互作用提出了挑战。我们调查了采用膜纳米光盘来容纳膜相关分子以应对挑战的可能性。纳米圆盘是盘状的稳定,均匀的膜片。它们被具有工程表位标签的环绕的两栖蛋白稳定。在本研究中,我们采用纳米光盘的抗原决定簇标签来检测和共免疫沉淀纳米光盘所含糖脂神经节苷脂GM1的相互作用伴侣。在来自产肠毒素的大肠埃希氏菌的培养基中,通过表面等离振子共振观察到了固定在传感器芯片上的纳米光盘-GM1的高特异性结合活性。为了从产肠毒素的大肠埃希氏菌中分离出相互作用伴侣,采用了GM1-nanodiscs进行共免疫沉淀。热不稳定肠毒素的B亚基已通过质谱鉴定为特定的相互作用伴侣,因此证明了纳米圆盘技术可用于高度特异性地检测和鉴定与嵌入双层膜中的特定脂质的相互作用伴侣。

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