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Rapid protein separation and diffusion coefficient measurement by frit inlet flow field-flow fractionation.

机译:通过熔块入口流场流分馏快速蛋白质分离和扩散系数测量。

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摘要

In this study three flow field-flow fractionation (flow FFF) channels are utilized for the separation of proteins and for the simultaneous measurement of their translational diffusion coefficients, D. One channel has a traditional sample inlet, whereas the other two incorporate a frit inlet design that permits more convenient and rapid sample introduction. The dependence of retention time on D, which leads to differential elution and the opportunity to measure D for protein peaks purified by the flow FFF process, is described theoretically and examined experimentally. Factors affecting band broadening, resolution, and optimization are also examined. The separation of proteins is achieved in the time range 4-20 min. Partial resolution is achieved in multiple runs requiring 2 min each. Values of D calculated from retention times are reported for 15 proteins. These include two protein dimers (bovine serum albumin and gamma-globulin) not ordinarily accessible to measurement. The D values from the three channels are compared with one another and with literature data. Reasonable consistency (within 3-4%) is found. High-speed repetitive runs can be used to acquire multiple values of D in time intervals as short as 1 min.
机译:在这项研究中,三个流场-流动分馏(flow FFF)通道用于分离蛋白质并同时测量其翻译扩散系数D。一个通道具有传统的样品入口,而另两个通道具有玻璃料入口允许更方便,更快速地引入样品的设计。保留时间对D的依赖性会导致差异洗脱,并为通过流动FFF过程纯化的蛋白质峰测量D的机会在理论上进行了描述并进行了实验检验。还检查了影响谱带展宽,分辨率和优化的因素。蛋白质的分离在4-20分钟的时间范围内完成。通过多次运行(每次需要2分钟)来实现部分分辨率。报告了从保留时间计算出的15种蛋白质的D值。其中包括通常无法测量的两个蛋白质二聚体(牛血清白蛋白和γ-球蛋白)。将三个通道的D值相互比较,并与文献数据进行比较。发现合理的一致性(3-4%之内)。高速重复运行可用于以短至1分钟的时间间隔获取多个D值。

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