Issue 10, 2017

Protein labeling for live cell fluorescence microscopy with a highly photostable renewable signal

Abstract

We present protein-PAINT – the implementation of the general principles of PAINT (Point Accumulation for Imaging in Nanoscale Topography) for live-cell protein labeling. Our method employs the specific binding of cell-permeable fluorogenic dyes to genetically encoded protein tags. We engineered three mutants of the bacterial lipocalin Blc that possess different affinities to a fluorogenic dye and exhibit a strong increase in fluorescence intensity upon binding. This allows for rapid labeling and washout of intracellular targets on a time scale from seconds to a few minutes. We demonstrate an order of magnitude higher photostability of the fluorescence signal in comparison with spectrally similar fluorescent proteins. Protein-PAINT ensures prolonged super-resolution fluorescence microscopy of living cells in both single molecule detection and stimulated emission depletion regimes.

Graphical abstract: Protein labeling for live cell fluorescence microscopy with a highly photostable renewable signal

Supplementary files

Article information

Article type
Edge Article
Submitted
11 Apr 2017
Accepted
01 Aug 2017
First published
03 Aug 2017
This article is Open Access

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

Chem. Sci., 2017,8, 7138-7142

Protein labeling for live cell fluorescence microscopy with a highly photostable renewable signal

N. G. Bozhanova, M. S. Baranov, N. V. Klementieva, K. S. Sarkisyan, A. S. Gavrikov, I. V. Yampolsky, E. V. Zagaynova, S. A. Lukyanov, K. A. Lukyanov and A. S. Mishin, Chem. Sci., 2017, 8, 7138 DOI: 10.1039/C7SC01628J

This article is licensed under a Creative Commons Attribution 3.0 Unported Licence. You can use material from this article in other publications without requesting further permissions from the RSC, provided that the correct acknowledgement is given.

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