Tracking protein turnover and degradation by microscopy: photo-switchable versus time-encoded fluorescent proteins

利用显微镜追踪蛋白质的周转和降解:光开关荧光蛋白与时间编码荧光蛋白

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Abstract

Expanded fluorescent protein techniques employing photo-switchable and fluorescent timer proteins have become important tools in biological research. These tools allow researchers to address a major challenge in cell and developmental biology, namely obtaining kinetic information about the processes that determine the distribution and abundance of proteins in cells and tissues. This knowledge is often essential for the comprehensive understanding of a biological process, and/or required to determine the precise point of interference following an experimental perturbation.

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