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Intrinsic blinking of red fluorescent proteins for super-resolution microscopy.

Natalia V Klementieva, Anton I Pavlikov, Alexander A Moiseev, Nina G Bozhanova, Natalie M Mishina, Sergey A Lukyanov, Elena V Zagaynova, Konstantin A Lukyanov, Alexander S Mishin
Chemical Communications : Chem Comm 2017 January 11
Single-molecule localization microscopy relies on either controllable photoswitching of fluorescent probes or their robust blinking. We have found that blinking of monomeric red fluorescent proteins TagRFP, TagRFP-T, and FusionRed occurs at moderate illumination power and matches well with camera acquisition speed. It allows for super-resolution image reconstruction of densely labelled structures in live cells using various algorithms.

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