Issue 21, 2024

Bioisostere-conjugated fluorescent probes for live-cell protein imaging without non-specific organelle accumulation

Abstract

Specific labeling of proteins using membrane-permeable fluorescent probes is a powerful technique for bioimaging. Cationic fluorescent dyes with high fluorescence quantum yield, photostability, and water solubility provide highly useful scaffolds for protein-labeling probes. However, cationic probes generally show undesired accumulation in organelles, which causes a false-positive signal in localization analysis. Herein, we report a design strategy for probes that suppress undesired organelle accumulation using a bioisostere for intracellular protein imaging in living cells. Our design allows the protein labeling probes to possess both membrane permeability and suppress non-specific accumulation and has been shown to use several protein labeling systems, such as PYP-tag and Halo tag systems. We further developed a fluorogenic PYP-tag labeling probe for intracellular proteins and used it to visualize multiple localizations of target proteins in the intracellular system. Our strategy offers a versatile design for undesired accumulation-suppressed probes with cationic dye scaffolds and provides a valuable tool for intracellular protein imaging.

Graphical abstract: Bioisostere-conjugated fluorescent probes for live-cell protein imaging without non-specific organelle accumulation

Supplementary files

Article information

Article type
Edge Article
Submitted
27 Dec 2023
Accepted
26 Apr 2024
First published
01 May 2024
This article is Open Access

All publication charges for this article have been paid for by the Royal Society of Chemistry
Creative Commons BY-NC license

Chem. Sci., 2024,15, 8097-8105

Bioisostere-conjugated fluorescent probes for live-cell protein imaging without non-specific organelle accumulation

T. Kamikawa, A. Hashimoto, N. Yamazaki, J. Adachi, A. Matsushima, K. Kikuchi and Y. Hori, Chem. Sci., 2024, 15, 8097 DOI: 10.1039/D3SC06957E

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