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用于毛细管凝胶电泳蛋白质分析的染色方法。

Staining method for protein analysis by capillary gel electrophoresis.

作者信息

Wu Shuqing, Lu Joann J, Wang Shili, Peck Kristy L, Li Guigen, Liu Shaorong

机构信息

Department of Chemistry and Biochemistry, Texas Tech University, Lubbock, Texas 79409, USA.

出版信息

Anal Chem. 2007 Oct 15;79(20):7727-33. doi: 10.1021/ac071055n. Epub 2007 Sep 18.

Abstract

A novel staining method and the associated fluorescent dye were developed for protein analysis by capillary SDS-PAGE. The method strategy is to synthesize a pseudo-SDS dye and use it to replace some of the SDS in SDS-protein complexes so that the protein can be fluorescently detected. The pseudo-SDS dye consists of a long, straight alkyl chain connected to a negative charged fluorescent head and binds to proteins just as SDS. The number of dye molecules incorporated with a protein depends on the dye concentration relative to SDS in the sample solution, since SDS and dye bind to proteins competitively. In this work, we synthesized a series of pseudo-SDS dyes, and tested their performances for capillary SDS-PAGE. FT-16 (a fluorescein molecule linked with a hexadodecyl group) seemed to be the best among all the dyes tested. Although the numbers of dye molecules bound to proteins (and the fluorescence signals from these protein complexes) were maximized in the absence of SDS, high-quality separations were obtained when co-complexes of SDS-protein-dye were formed. The migration time correlates well with protein size even after some of the SDS in the SDS-protein complexes was replaced by the pseudo-SDS dye. Under optimized experimental conditions and using a laser-induced fluorescence detector, limits of detection of as low as 0.13 ng/mL (bovine serum albumin) and dynamic ranges over 5 orders of magnitude in which fluorescence response is proportional to the square root of analyte concentration were obtained. The method and dye were also tested for separations of real-world samples from E. coli.

摘要

开发了一种用于毛细管SDS-PAGE蛋白质分析的新型染色方法及相关荧光染料。该方法策略是合成一种假SDS染料,并用它取代SDS-蛋白质复合物中的部分SDS,从而实现蛋白质的荧光检测。假SDS染料由连接到带负电荷荧光头的长直烷基链组成,与SDS一样能与蛋白质结合。结合到蛋白质上的染料分子数量取决于样品溶液中染料相对于SDS的浓度,因为SDS和染料竞争性地与蛋白质结合。在这项工作中,我们合成了一系列假SDS染料,并测试了它们在毛细管SDS-PAGE中的性能。FT-16(一种与十六烷基相连的荧光素分子)似乎是所有测试染料中效果最好的。尽管在没有SDS的情况下,结合到蛋白质上的染料分子数量(以及这些蛋白质复合物的荧光信号)达到最大值,但当形成SDS-蛋白质-染料的共复合物时,仍能获得高质量的分离效果。即使SDS-蛋白质复合物中的部分SDS被假SDS染料取代,迁移时间与蛋白质大小仍有良好的相关性。在优化的实验条件下,使用激光诱导荧光检测器,检测限低至0.13 ng/mL(牛血清白蛋白),动态范围超过5个数量级,其中荧光响应与分析物浓度的平方根成正比。该方法和染料还用于分离来自大肠杆菌的实际样品的测试。

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