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生色团辅助激光灭活

Chromophore-assisted laser inactivation.

作者信息

Hoffman-Kim Diane, Diefenbach Thomas J, Eustace Brenda K, Jay Daniel G

机构信息

Department of Molecular Pharmacology, Physiology, and Biotechnology, Center for Biomedical Engineering, Brown University, Providence, Rhode Island 02912, USA.

出版信息

Methods Cell Biol. 2007;82:335-54. doi: 10.1016/S0091-679X(06)82011-X.

Abstract

The major challenge of the post-genome world is ascribing in situ function to the myriad of proteins expressed in the proteome. This challenge is met by an arsenal of inactivation strategies that include RNAi and genetic knockout. These are powerful approaches but are indirect with respect to protein function and are subject to time delays before onset and possible genetic compensation. This chapter describes two protein-based inactivation approaches called chromophore-assisted laser inactivation (CALI) and fluorophore-assisted light inactivation (FALI). For CALI and FALI, light inactivation is targeted via photosensitizers that are localized to proteins of interest through antibody binding or expressed domains that are fluorescent or bind fluorescent probes. Inactivation occurs when and where the cells or tissues are irradiated and thus CALI and FALI provide an unprecedented level of spatial and temporal resolution of protein inactivation. Here we provide methods for the labeling of antibodies and setup of light sources and discuss controls, advantages of the technology, and potential pitfalls. We conclude with a discussion on a number of new technologies derived from CALI that combine molecular genetic approaches with light-induced inactivation that provide new tools to address in situ protein function.

摘要

后基因组时代的主要挑战是确定蛋白质组中表达的无数蛋白质的原位功能。一系列包括RNA干扰和基因敲除在内的失活策略应对了这一挑战。这些都是强大的方法,但就蛋白质功能而言是间接的,并且在起效前存在时间延迟以及可能的基因补偿。本章介绍了两种基于蛋白质的失活方法,即发色团辅助激光失活(CALI)和荧光团辅助光失活(FALI)。对于CALI和FALI,光失活是通过光敏剂靶向的,这些光敏剂通过抗体结合或荧光或结合荧光探针的表达结构域定位于感兴趣的蛋白质上。当细胞或组织受到照射时,失活就会在此时此地发生,因此CALI和FALI提供了前所未有的蛋白质失活时空分辨率水平。在这里,我们提供了抗体标记和光源设置的方法,并讨论了对照、该技术的优点和潜在陷阱。我们最后讨论了一些源自CALI的新技术,这些技术将分子遗传学方法与光诱导失活相结合,提供了新的工具来研究原位蛋白质功能。

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