Reversible Live‐Cell Labeling with Retro‐engineered HaloTags Enables Long‐Term High‐ and Super‐Resolution Imaging

Author:

Holtmannspötter Michael1ORCID,Wienbeuker Eike1,Dellmann Timo2ORCID,Watrinet Isabelle1,Garcia‐Sáez Ana J.2ORCID,Johnsson Kai3ORCID,Kurre Rainer1ORCID,Piehler Jacob1ORCID

Affiliation:

1. Department of Biology/Chemistry and Center for Cellular Nanoanalytics Osnabrück University Barbarastraße 11 49076 Osnabrück Germany

2. Institute for Genetics and Cologne Excellence Cluster on Cellular Stress Responses in Aging-Associated Diseases (CECAD) University of Cologne Joseph-Stelzmann-Straße 26 50931 Cologne Germany

3. Department of Chemical Biology Max Planck Institute for Medical Research Jahnstraße 29 69120 Heidelberg Germany

Abstract

AbstractSelf‐labeling enzymes (SLE) such as the HaloTag have emerged as powerful tools in high and super‐resolution fluorescence microscopy. Newly developed fluorogenic SLE substrates enable imaging in the presence of excess dye. To exploit this feature for reversible labeling, we engineered two variants of HaloTag7 with restored dehalogenase activity. Kinetic studies in vitro showed different turnover kinetics for reHaloTagS (≈0.006 s−1) and reHaloTagF (≈0.055 s−1). Imaging by confocal and stimulated emission depletion microscopy yielded 3‐5‐time enhanced photostability of reHaloTag labeling. Prominently, single molecule imaging with reHaloTags enabled controlled and stable labeling density over extended time periods. By combination with structured illumination, simultaneous visualization of single molecule diffusion and organellar dynamics was achieved. These applications highlight the potential of reHaloTag labeling for pushing the limits of advanced fluorescence microscopy techniques.

Funder

Deutsche Forschungsgemeinschaft

Publisher

Wiley

Subject

General Chemistry,Catalysis

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