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Supported Bilayer Electrophoresis under Controlled Buffer Conditions

机译:在受控缓冲液条件下支持的双层电泳

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A pH controlled flow cell device was constructed to allow electrophoretic movement of charged lipids and membrane associated proteins in supported phospholipid bilayers. The device isolated electrolysis products near the electrodes from the electrophoresis process within the bilayer. This allowed the pH over the bilayer region to remain within +-0.2 pH units or better over many hours at salt concentrations up to 10 mM. Using this setup, it was found that the electrophoretic mobility of a dye conjugated lipid (Texas Red 1,2-dihexadecanoyl-sn-glycero-3-phosphoethanolamine (TR-DHPE)) was essentially constant between pH 3.3 and 9.3. In contrast, streptavidin, which was bound to biotinylated lipids, shifted from migrating cathodically at acidic pH values to migrating anodically under basic conditions. This shift was due to the modulation of the net charge on the protein, which changed the electrophoretic forces experienced by the macromolecule. The addition of a polyethylene glycol (PEG) cushion beneath the bilayer or the increase in the ionic strength of the buffer solution resulted in a decrease of the electroosmotic force experienced by the streptavidin with little effect on the Texas Red-DHPE. As such, it was possible in part to control the electrophoretic and electroosmotic contributions to streptavidin independently of one another.
机译:构造了pH控制的流通池设备,以使带电的脂质和与膜相关的蛋白质在支持的磷脂双层中进行电泳运动。该装置从双层内的电泳过程中分离出电极附近的电解产物。在盐浓度高达10 mM的情况下,这可以使双层区域的pH值在多个小时内保持在+ -0.2 pH单位以内,甚至更好。使用这种设置,发现染料共轭脂质(得克萨斯红1,2-二十六烷酰基-sn-甘油-3-磷酸乙醇胺(TR-DHPE))的电泳迁移率在pH 3.3和9.3之间基本恒定。相反,与生物素化脂质结合的抗生蛋白链菌素从在碱性pH值下阴极迁移到在碱性条件下阳极迁移。这种变化是由于蛋白质上净电荷的调节,从而改变了大分子所经历的电泳力。在双层下面添加聚乙二醇(PEG)缓冲垫或增加缓冲溶液的离子强度会导致链霉亲和素所经历的电渗力降低,而对德克萨斯红DHPE的影响很小。这样,可以部分独立地控制对链霉亲和素的电泳和电渗作用。

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