Single-molecule binding experiments on long time scales | Zendy

Mark P. Elenko | Zendy; Jack W. Szostak | Zendy; Antoine M. van Oijen | Zendy

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Single-molecule binding experiments on long time scales

Author(s) -

Mark P. Elenko,

Jack W. Szostak,

Antoine M. van Oijen

Publication year - 2010

Publication title -

review of scientific instruments

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.605

H-Index - 165

eISSN - 1089-7623

pISSN - 0034-6748

DOI - 10.1063/1.3473936

Subject(s) - photobleaching , total internal reflection fluorescence microscope , molecule , materials science , fluorescence recovery after photobleaching , kinetics , chemical physics , biological system , optics , fluorescence , microscopy , nanotechnology , chemistry , physics , organic chemistry , quantum mechanics , biology

We describe an approach for performing single-molecule binding experiments on time scales from hours to days, allowing for the observation of slower kinetics than have been previously investigated by single-molecule techniques. Total internal reflection fluorescence microscopy is used to image the binding of labeled ligand to molecules specifically coupled to the surface of an optically transparent flow cell. Long-duration experiments are enabled by ensuring sufficient positional, chemical, thermal, and image stability. Principal components of this experimental stability include illumination timing, solution replacement, and chemical treatment of solution to reduce photodamage and photobleaching; and autofocusing to correct for spatial drift.

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