Despite the great importance of membrane proteins, structural and functional studies of these proteins present major challenges. A significant hurdle is the extraction of the functional protein from its natural lipid membrane. Traditionally achieved with detergents, purification procedures can be costly and time consuming. A critical flaw with detergent approaches is the removal of the protein from the native lipid environment required to maintain functionally stable protein. This protocol describes the preparation of styrene maleic acid (SMA) co-polymer to extract membrane proteins from prokaryotic and eukaryotic expression systems. Successful isolation of membrane proteins into SMA lipid particles (SMALPs) allows the proteins to remain with native lipid, surrounded by SMA. We detail procedures for obtaining 25 g of SMA (4 d); explain the preparation of protein-containing SMALPs using membranes isolated from Escherichia coli (2 d) and control protein-free SMALPS using E. coli polar lipid extract (1–2 h); investigate SMALP protein purity by SDS–PAGE analysis and estimate protein concentration (4 h); and detail biophysical methods such as circular dichroism (CD) spectroscopy and sedimentation velocity analytical ultracentrifugation (svAUC) to undertake initial structural studies to characterize SMALPs (~2 d). Together, these methods provide a practical tool kit for those wanting to use SMALPs to study membrane proteins.
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机译:尽管膜蛋白非常重要,但对这些蛋白的结构和功能研究仍存在重大挑战。一个重要的障碍是从其天然脂质膜中提取功能蛋白。传统上用洗涤剂实现,纯化过程可能既昂贵又费时。去污剂方法的一个关键缺陷是从维持功能上稳定的蛋白质所需的天然脂质环境中去除蛋白质。该协议描述了制备苯乙烯马来酸(SMA)共聚物以从原核和真核表达系统中提取膜蛋白的方法。将膜蛋白成功分离成SMA脂质颗粒(SMALP),可使蛋白与天然脂质一起保留,并被SMA包围。我们详细介绍了获得25 g SMA(4 d)的程序。解释使用从大肠杆菌分离的膜制备含蛋白质的SMALP(2天),并使用大肠杆菌极性脂质提取物(1-2小时)控制无蛋白质的SMALPS;通过SDS-PAGE分析研究SMALP蛋白的纯度,并估计蛋白浓度(4小时);并详细介绍了生物物理方法,例如圆二色性(CD)光谱和沉降速度分析超速离心(svAUC),以进行初步的结构研究来表征SMALP(约2 d)。总之,这些方法为那些希望使用SMALP研究膜蛋白的人提供了实用的工具套件。
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