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

被引:58
作者
Bozhanova, Nina G. [1 ,2 ]
Baranov, Mikhail S. [1 ]
Klementieva, Natalia V. [2 ]
Sarkisyan, Karen S. [1 ,3 ]
Gavrikov, Alexey S. [1 ]
Yampolsky, Ilia V. [1 ,4 ]
Zagaynova, Elena V. [2 ]
Lukyanov, Sergey A. [1 ,2 ,4 ]
Lukyanov, Konstantin A. [1 ,2 ]
Mishin, Alexander S. [1 ,2 ]
机构
[1] Shemyakin Ovchinnikov Inst Bioorgan Chem, Moscow, Russia
[2] Nizhny Novgorod State Med Acad, Nizhnii Novgorod, Russia
[3] Barcelona Inst Sci & Technol, Ctr Genom Regulat CRG, Dr Aiguader 88, Barcelona 08003, Spain
[4] Pirogov Russian Natl Res Med Univ, Moscow, Russia
基金
俄罗斯科学基金会;
关键词
LIVING CELLS; GFP CHROMOPHORE; SUPERRESOLUTION MICROSCOPY; LOCALIZATION MICROSCOPY; FLUOROPHORE LIGASE; DIRECTED EVOLUTION; FLUOROGENIC PROBES; BINDING; EXCHANGE; TAG;
D O I
10.1039/c7sc01628j
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
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.
引用
收藏
页码:7138 / 7142
页数:5
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