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Surpassing the lateral resolution limit by a factor of two using structured illumination microscopy

SHORT COMMUNICATION

M. G. L. Gustafsson

Department of Biochemistry and Biophysics, University of California San Francisco,
San Francisco, California 94143‐0448, U.S.A.

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First published: 24 December 2001
Cited by: 1079
M. G. L. Gustafsson. Tel: + 1 415 476 2489; fax: + 1 415 476 1902; e‐mail: mats@msg.ucsf.edu

Abstract

Lateral resolution that exceeds the classical diffraction limit by a factor of two is achieved by using spatially structured illumination in a wide‐field fluorescence microscope. The sample is illuminated with a series of excitation light patterns, which cause normally inaccessible high‐resolution information to be encoded into the observed image. The recorded images are linearly processed to extract the new information and produce a reconstruction with twice the normal resolution. Unlike confocal microscopy, the resolution improvement is achieved with no need to discard any of the emission light. The method produces images of strikingly increased clarity compared to both conventional and confocal microscopes.

Number of times cited: 1079

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