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使用可细胞渗透且可裂解的氯代烷烃衍生化小分子进行靶点鉴定

Target Identification Using Cell Permeable and Cleavable Chloroalkane Derivatized Small Molecules.

作者信息

Mendez-Johnson Jacqui L, Daniels Danette L, Urh Marjeta, Friedman Ohana Rachel

机构信息

Promega Corporation, 2800 Woods Hollow Rd, Madison, WI, 53711, USA.

出版信息

Methods Mol Biol. 2017;1647:91-108. doi: 10.1007/978-1-4939-7201-2_6.

Abstract

An important aspect for gaining functional insight into the activity of small molecules revealed through phenotypic screening is the identification of their interacting proteins. Yet, isolating and validating these interacting proteins remains difficult. Here, we present a new approach utilizing a chloroalkane (CA) moiety capture handle, which can be chemically attached to small molecules to isolate their respective protein targets. Derivatization of small molecules with the CA moiety has been shown to not significantly impact their cell permeability or potency, allowing for phenotypic validation of the derivatized small molecule prior to capture. The retention of cell permeability also allows for treatment of live cells with the derivatized small molecule and the CA moiety enables rapid covalent capture onto HaloTag coated magnetic beads. Additionally, several options are available for the elution of interacting proteins, including chemical cleavage of the CA moiety, competitive elution using excess unmodified small molecule, or sodium dodecyl sulfate (SDS) elution. These features taken together yield a highly robust and efficient process for target identification, including capture of weak or low abundance interactors.

摘要

通过表型筛选揭示的小分子活性,深入了解其功能的一个重要方面是识别与之相互作用的蛋白质。然而,分离和验证这些相互作用的蛋白质仍然很困难。在这里,我们提出了一种利用氯代烷烃(CA)部分捕获手柄的新方法,该手柄可以化学连接到小分子上,以分离它们各自的蛋白质靶点。已证明用CA部分对小分子进行衍生化不会显著影响其细胞通透性或效力,从而可以在捕获之前对衍生化的小分子进行表型验证。细胞通透性的保留还允许用衍生化的小分子处理活细胞,并且CA部分能够快速共价捕获到HaloTag包被的磁珠上。此外,有几种洗脱相互作用蛋白质的方法可供选择,包括CA部分的化学裂解、使用过量未修饰小分子的竞争性洗脱或十二烷基硫酸钠(SDS)洗脱。这些特性共同产生了一个高度稳健和高效的靶点识别过程,包括捕获弱或低丰度的相互作用分子。

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