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Protein Separation by Electrophoretic-Electroosmotic Focusing on Supported Lipid Bilayers

机译:电泳-电渗流法聚焦于支持脂质双层的蛋白质分离

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摘要

An electrophoretic-electroosmotic focusing (EEF) method was developed and used to separate membrane-bound proteins and charged lipids based on their charge-to-size ratio from an initially homogeneous mixture. EEF uses opposing electrophoretic and electroosmotic forces to focus and separate proteins and lipids into narrow bands on supported lipid bilayers (SLBs). Membrane-associated species were focused into specific positions within the SLB in a highly repeatable fashion. The steady-state focusing positions of the proteins could be predicted and controlled by tuning experimental conditions, such as buffer pH, ionic strength, electric field, and temperature. Careful tuning of the variables should enable one to separate mixtures of membrane proteins with only subtle differences. The EEF technique was found to be an effective way to separate protein mixtures with low initial concentrations, and it overcame diffusive peak broadening to allow four bands to be separated simultaneously within a 380 (mu)m wide isolated supported membrane patch.
机译:电泳-电渗聚焦(EEF)方法得到了发展,并用于从最初均质的混合物中根据膜与蛋白和带电脂质的电荷-尺寸比来分离它们。 EEF使用相反的电泳和电渗力将蛋白质和脂质聚焦并分离为支持的脂质双层(SLB)上的窄带。膜相关物种以高度可重复的方式集中到SLB中的特定位置。蛋白质的稳态聚焦位置可以通过调整实验条件(例如缓冲液pH值,离子强度,电场和温度)来预测和控制。仔细调整变量应能使膜蛋白的混合物仅具有细微的差异。发现EEF技术是分离低初始浓度蛋白质混合物的有效方法,它克服了扩散峰展宽的问题,可以在380μm宽的分离的支持膜贴片中同时分离出四个谱带。

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