首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >Proteinase assay by capillary electrophoresis employing fluorescence-quenched protein-dye conjugates
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Proteinase assay by capillary electrophoresis employing fluorescence-quenched protein-dye conjugates

机译:使用荧光猝灭的蛋白质染料偶联物通过毛细管电泳进行蛋白酶测定

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Determination of proteinases - enzymes that catalyze the hydrolysis of peptide bonds - is often difficult due to the presence of interferences in complex biological media and limited sample size. Capillary electrophoresis (CE), with laser-induced fluorescence (LIF) can serve as a useful tool for such determinations. LIF detection offers the advantages of increased sensitivity and increased selectivity. However, direct LIF detection requires the proteinase analyte to be fluorescently derivatized prior to analysis. A viable alternative is offered by the present work, in which protein substrates are first labeled with BODIPY dye, a relatively pH-insensitive, high-fluorescence quantum yield dye. Upon binding of some 4-10 molecules of dye to a single protein, the dye is effectively fluorescence-quenched. Digestion of the BODIPY - labeled and quenched protein by an unlabeled enzyme yields smaller peptide fragments in which the fluorescence of associated BODIPY tags is restored. We will present how the fragmentation pattern of BODIPY-labeled casein changes as a function of incubation time with trypsin, as well as the effect of varying concentrations of trypsin on the BODIPY-casein digest. [References: 27]
机译:由于复杂的生物介质中存在干扰并且样品量有限,蛋白酶(一种催化肽键水解的酶)的测定通常很困难。毛细管电泳(CE)和激光诱导的荧光(LIF)可以用作此类测定的有用工具。 LIF检测具有提高灵敏度和提高选择性的优势。但是,直接LIF检测需要在分析之前将蛋白酶分析物进行荧光衍生。本工作提供了一种可行的替代方法,其中首先用BODIPY染料标记蛋白质底物,BODIPY染料是一种对pH值不敏感的高荧光量子产率染料。在将约4-10个分子的染料与单个蛋白质结合后,该染料将被有效地荧光猝灭。用未标记的酶消化BODIPY标记和淬灭的蛋白质会产生较小的肽片段,其中相关的BODIPY标签的荧光得以恢复。我们将介绍BODIPY标记的酪蛋白的片段化模式如何随胰蛋白酶孵育时间的变化而变化,以及不同浓度的胰蛋白酶对BODIPY-酪蛋白消化物的影响。 [参考:27]

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