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Two-dimensional capillary electrophoresis: Capillary isoelectric focusing and capillary zone electrophoresis with laser-induced fluorescence detection

机译:二维毛细管电泳:毛细管等电聚焦和毛细管区带激光诱导荧光检测

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摘要

CIEF and CZE are coupled with LIF detection to create an ultrasensitive 2-D separation method for proteins. In this method, two capillaries are joined through a buffer-filled interface. Separate power supplies control the potential at the injection end of the first capillary and at the interface; the detector is held at ground potential. Proteins are labeled with the fluorogenic reagent Chromeo P503, which preserves the isoelectric point of the labeled protein. The labeled proteins were mixed with ampholytes and injected into the first-dimension capillary. A focusing step was performed with the injection end of the capillary at high pH and the interface at low pH. To mobilize components, the interface was filled with a high pH buffer, which was compatible with the second-dimension separation. A fraction was transferred to the second-dimension capillary for separation. The process of fraction transfer and second dimension separation was repeated two dozen times. The separation produced a spot capacity of 125.
机译:CIEF和CZE与LIF检测结合使用,可为蛋白质创建超灵敏的二维分离方法。在这种方法中,两个毛细管通过缓冲液填充的接口相连。独立的电源控制着第一个毛细管的注射端和界面处的电势;检测器保持在地电位。蛋白用荧光试剂Chromeo P503标记,该试剂保留了标记蛋白的等电点。将标记的蛋白质与两性电解质混合,并注入第一维毛细管中。聚焦步骤是在毛细管的注射端处于高pH值而界面处于低pH值的条件下进行的。为了调动组件,在界面中填充了高pH缓冲液,该缓冲液与第二维分离兼容。将馏分转移至第二维毛细管进行分离。馏分转移和第二维分离的过程重复两次。分离产生的点容量为125。

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