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一种用于在活细胞中对蛋白质进行翻译后标记以进行荧光成像和追踪的新方法。

A new method for post-translationally labeling proteins in live cells for fluorescence imaging and tracking.

作者信息

Hinrichsen M, Lenz M, Edwards J M, Miller O K, Mochrie S G J, Swain P S, Schwarz-Linek U, Regan L

机构信息

Department of Molecular Biophysics and Biochemistry, Yale University, 266 Whitney Avenue, New Haven, CT06511, USA.

SynthSys-Synthetic and Systems Biology, School of Biological Sciences, University of Edinburgh, Edinburgh EH9 3BF, UK.

出版信息

Protein Eng Des Sel. 2017 Dec 1;30(12):771-780. doi: 10.1093/protein/gzx059.

Abstract

We present a novel method to fluorescently label proteins, post-translationally, within live Saccharomycescerevisiae. The premise underlying this work is that fluorescent protein (FP) tags are less disruptive to normal processing and function when they are attached post-translationally, because target proteins are allowed to fold properly and reach their final subcellular location before being labeled. We accomplish this post-translational labeling by expressing the target protein fused to a short peptide tag (SpyTag), which is then covalently labeled in situ by controlled expression of an open isopeptide domain (SpyoIPD, a more stable derivative of the SpyCatcher protein) fused to an FP. The formation of a covalent bond between SpyTag and SpyoIPD attaches the FP to the target protein. We demonstrate the general applicability of this strategy by labeling several yeast proteins. Importantly, we show that labeling the membrane protein Pma1 in this manner avoids the mislocalization and growth impairment that occur when Pma1 is genetically fused to an FP. We also demonstrate that this strategy enables a novel approach to spatiotemporal tracking in single cells and we develop a Bayesian analysis to determine the protein's turnover time from such data.

摘要

我们提出了一种在活的酿酒酵母中对蛋白质进行翻译后荧光标记的新方法。这项工作的基本前提是,荧光蛋白(FP)标签在翻译后附着时对正常加工和功能的干扰较小,因为目标蛋白在被标记之前能够正确折叠并到达其最终的亚细胞位置。我们通过表达与短肽标签(SpyTag)融合的目标蛋白来实现这种翻译后标记,然后通过与FP融合的开放异肽结构域(SpyoIPD,SpyCatcher蛋白的更稳定衍生物)的可控表达在原位进行共价标记。SpyTag和SpyoIPD之间形成共价键将FP连接到目标蛋白上。我们通过标记几种酵母蛋白证明了该策略的普遍适用性。重要的是,我们表明以这种方式标记膜蛋白Pma1可避免当Pma1与FP进行基因融合时出现的错误定位和生长受损。我们还证明了该策略能够实现单细胞中的时空追踪新方法,并且我们开发了一种贝叶斯分析方法来从此类数据确定蛋白质的周转时间。

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