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首页> 外文期刊>Frontiers in Microbiology >Utilizing Biotinylated Proteins Expressed in Yeast to Visualize DNA–Protein Interactions at the Single-Molecule Level
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Utilizing Biotinylated Proteins Expressed in Yeast to Visualize DNA–Protein Interactions at the Single-Molecule Level

机译:利用酵母中表达的生物素化蛋白在单分子水平上可视化DNA-蛋白质相互作用。

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Much of our knowledge in conventional biochemistry has derived from bulk assays. However, many stochastic processes and transient intermediates are hidden when averaged over the ensemble. The powerful technique of single-molecule fluorescence microscopy has made great contributions to the understanding of life processes that are inaccessible when using traditional approaches. In single-molecule studies, quantum dots (Qdots) have several unique advantages over other fluorescent probes, such as high brightness, extremely high photostability, and large Stokes shift, thus allowing long-time observation and improved signal-to-noise ratios. So far, however, there is no convenient way to label proteins purified from budding yeast with Qdots. Based on BirA–Avi and biotin–streptavidin systems, we have established a simple method to acquire a Qdot-labeled protein and visualize its interaction with DNA using total internal reflection fluorescence microscopy. For proof-of-concept, we chose replication protein A (RPA) and origin recognition complex (ORC) as the proteins of interest. Proteins were purified from budding yeast with high biotinylation efficiency and rapidly labeled with streptavidin-coated Qdots. Interactions between proteins and DNA were observed successfully at the single-molecule level.
机译:我们在常规生物化学中的许多知识都来自批量测定。但是,对整个集合求平均时,许多随机过程和瞬态中间体会被隐藏。强大的单分子荧光显微镜技术为理解使用传统方法无法达到的生命过程做出了巨大贡献。在单分子研究中,量子点(Qdots)与其他荧光探针相比具有一些独特的优势,例如高亮度,极高的光稳定性和大的斯托克斯位移,从而可以进行长时间观察并改善信噪比。但是,到目前为止,还没有方便的方法来用Qdots标记从发芽酵母中纯化的蛋白质。基于BirA-Avi和生物素-链霉亲和素系统,我们建立了一种简单的方法来获取Qdot标记的蛋白质,并使用全内反射荧光显微镜观察其与DNA的相互作用。为了进行概念验证,我们选择复制蛋白A(RPA)和起源识别复合物(ORC)作为目标蛋白。从出芽的酵母中纯化出具有高生物素化效率的蛋白质,并用链霉亲和素包被的Qdots快速标记。在单分子水平成功观察到蛋白质和DNA之间的相互作用。

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