Thimon Véronique, Belghazi Maya, Labas Valérie, Dacheux Jean-Louis, Gatti Jean-Luc
Gamètes Males et Fertilité, INRA, CNRS, Haras Nationaux, Université de Tours, Institut National de la Recherche Agronomique, Station de Physiologie de la Reproduction et des Comportements, 37380 Nouzilly, France.
Anal Biochem. 2008 Apr 15;375(2):382-4. doi: 10.1016/j.ab.2007.12.026. Epub 2007 Dec 25.
We describe a simple and direct zymographic method for the detection of proteases using quenched fluorescent substrates. The proteases were separated using one- and two-dimensional electrophoresis, and the gel subsequently was incubated with the quenched fluorescent substrate. After a short incubation, the released fluorescence allowed the localization of the proteases directly using UV light. The protease spots could then be cut directly from the gel and processed for identification by mass spectrometry. This method could easily be used to develop or test whether a substrate is specific or not and also to detect the proteases that are able to cleave this substrate in a complex biological fluid. This also allowed direct identification of proteases without complex purification.
我们描述了一种使用淬灭荧光底物检测蛋白酶的简单直接的酶谱法。通过一维和二维电泳分离蛋白酶,随后将凝胶与淬灭荧光底物一起孵育。短暂孵育后,释放的荧光使得能够直接使用紫外光对蛋白酶进行定位。然后可以直接从凝胶上切下蛋白酶斑点,并进行处理以通过质谱鉴定。该方法可轻松用于开发或测试底物是否具有特异性,还可用于检测能够在复杂生物流体中切割该底物的蛋白酶。这也使得无需复杂纯化即可直接鉴定蛋白酶。
