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基于蛋白水解切割的膜转位分析:应用于白喉毒素T结构域

Membrane translocation assay based on proteolytic cleavage: application to diphtheria toxin T domain.

作者信息

Rodnin Mykola V, Ladokhin Alexey S

机构信息

Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, KS 66160, United States.

Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, KS 66160, United States.

出版信息

Biochim Biophys Acta. 2015 Jan;1848(1 Pt A):35-40. doi: 10.1016/j.bbamem.2014.09.013. Epub 2014 Oct 5.

Abstract

The function of diphtheria toxin translocation (T) domain is to transfer the catalytic domain across the endosomal membrane upon acidification. The goal of this study was to develop and apply an in vitro functional assay for T domain activity, suitable for investigation of structure-function relationships of translocation across lipid bilayers of various compositions. Traditionally, T domain activity in vitro is estimated by measuring either conductance in planar lipid bilayers or the release of fluorescent markers from lipid vesicles. While an in vivo cell death assay is the most relevant to physiological function, it cannot be applied to studying the effects of pH or membrane lipid composition on translocation. Here we suggest an assay based on cleavage of the N-terminal part of T domain upon translocation into protease-loaded vesicles. A series of control experiment was used to confirm that cleavage occurs inside the vesicle and not as the result of vesicle disruption. Translocation of the N-terminus of the T domain is shown to require the presence of a critical fraction of anionic lipids, which is consistent with our previous biophysical measurements of insertion. Application of the proposed assay to a series of T domain mutants correlated well with the results of cytotoxicity assay.

摘要

白喉毒素转位(T)结构域的功能是在酸化时将催化结构域转运穿过内体膜。本研究的目的是开发并应用一种用于T结构域活性的体外功能测定法,该方法适用于研究跨各种组成的脂质双层转位的结构-功能关系。传统上,体外T结构域活性通过测量平面脂质双层中的电导或脂质囊泡中荧光标记物的释放来估计。虽然体内细胞死亡测定与生理功能最相关,但它不能用于研究pH或膜脂质组成对转位的影响。在此,我们提出一种基于T结构域N端部分在转位到装载蛋白酶的囊泡中时被切割的测定法。一系列对照实验用于证实切割发生在囊泡内部,而不是囊泡破裂的结果。T结构域N端的转位显示需要一定比例的关键阴离子脂质,这与我们之前关于插入的生物物理测量结果一致。将所提出的测定法应用于一系列T结构域突变体,其结果与细胞毒性测定结果相关性良好。

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