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Literature DB >> 18326650

Three-dimensional resolution doubling in wide-field fluorescence microscopy by structured illumination.

Mats G L Gustafsson¹, Lin Shao, Peter M Carlton, C J Rachel Wang, Inna N Golubovskaya, W Zacheus Cande, David A Agard, John W Sedat.

Abstract

Structured illumination microscopy is a method that can increase the spatial resolution of wide-field fluorescence microscopy beyond its classical limit by using spatially structured illumination light. Here we describe how this method can be applied in three dimensions to double the axial as well as the lateral resolution, with true optical sectioning. A grating is used to generate three mutually coherent light beams, which interfere in the specimen to form an illumination pattern that varies both laterally and axially. The spatially structured excitation intensity causes normally unreachable high-resolution information to become encoded into the observed images through spatial frequency mixing. This new information is computationally extracted and used to generate a three-dimensional reconstruction with twice as high resolution, in all three dimensions, as is possible in a conventional wide-field microscope. The method has been demonstrated on both test objects and biological specimens, and has produced the first light microscopy images of the synaptonemal complex in which the lateral elements are clearly resolved.

Mesh：

Year: 2008 PMID： 18326650 PMCID： PMC2397368 DOI： 10.1529/biophysj.107.120345

Source DB: PubMed Journal: Biophys J ISSN： 0006-3495 Impact factor: 4.033

23 in total

1. I5M: 3D widefield light microscopy with better than 100 nm axial resolution.

Authors: M G Gustafsson; D A Agard; J W Sedat
Journal: J Microsc Date: 1999-07 Impact factor: 1.758

2. True optical resolution beyond the Rayleigh limit achieved by standing wave illumination.

Authors: J T Frohn; H F Knapp; A Stemmer
Journal: Proc Natl Acad Sci U S A Date: 2000-06-20 Impact factor: 11.205

3. Saturated patterned excitation microscopy--a concept for optical resolution improvement.

Authors: Rainer Heintzmann; Thomas M Jovin; Christoph Cremer
Journal: J Opt Soc Am A Opt Image Sci Vis Date: 2002-08 Impact factor: 2.129

4. Wide-field subdiffraction RESOLFT microscopy using fluorescent protein photoswitching.

Authors: Miriam A Schwentker; Hannes Bock; Michael Hofmann; Stefan Jakobs; Jörg Bewersdorf; Christian Eggeling; Stefan W Hell
Journal: Microsc Res Tech Date: 2007-03 Impact factor: 2.769

5. Three-dimensional resolution enhancement in fluorescence microscopy by harmonic excitation.

Authors: J T Frohn; H F Knapp; A Stemmer
Journal: Opt Lett Date: 2001-06-01 Impact factor: 3.776

6. Two-dimensional standing wave total internal reflection fluorescence microscopy: superresolution imaging of single molecular and biological specimens.

Authors: Euiheon Chung; Daekeun Kim; Yan Cui; Yang-Hyo Kim; Peter T C So
Journal: Biophys J Date: 2007-05-04 Impact factor: 4.033

7. Direct evidence of a role for heterochromatin in meiotic chromosome segregation.

Authors: A F Dernburg; J W Sedat; R S Hawley
Journal: Cell Date: 1996-07-12 Impact factor: 41.582

Review 8. Fluorescence microscopy in three dimensions.

Authors: D A Agard; Y Hiraoka; P Shaw; J W Sedat
Journal: Methods Cell Biol Date: 1989 Impact factor: 1.441

9. Asy1, a protein required for meiotic chromosome synapsis, localizes to axis-associated chromatin in Arabidopsis and Brassica.

Authors: Susan J Armstrong; Anthony P Caryl; Gareth H Jones; F Christopher H Franklin
Journal: J Cell Sci Date: 2002-09-15 Impact factor: 5.285

10. The pam1 gene is required for meiotic bouquet formation and efficient homologous synapsis in maize (Zea mays L.).

Authors: Inna N Golubovskaya; Lisa C Harper; Wojciech P Pawlowski; Denise Schichnes; W Zacheus Cande
Journal: Genetics Date: 2002-12 Impact factor: 4.562

458 in total

1. Nonlinear structured-illumination microscopy with a photoswitchable protein reveals cellular structures at 50-nm resolution.

Authors: E Hesper Rego; Lin Shao; John J Macklin; Lukman Winoto; Göran A Johansson; Nicholas Kamps-Hughes; Michael W Davidson; Mats G L Gustafsson
Journal: Proc Natl Acad Sci U S A Date: 2011-12-12 Impact factor: 11.205

Three-dimensional resolution doubling in wide-field fluorescence microscopy by structured illumination.

1. I5M: 3D widefield light microscopy with better than 100 nm axial resolution.

2. True optical resolution beyond the Rayleigh limit achieved by standing wave illumination.

3. Saturated patterned excitation microscopy--a concept for optical resolution improvement.

4. Wide-field subdiffraction RESOLFT microscopy using fluorescent protein photoswitching.

5. Three-dimensional resolution enhancement in fluorescence microscopy by harmonic excitation.

6. Two-dimensional standing wave total internal reflection fluorescence microscopy: superresolution imaging of single molecular and biological specimens.

7. Direct evidence of a role for heterochromatin in meiotic chromosome segregation.

Review 8. Fluorescence microscopy in three dimensions.

9. Asy1, a protein required for meiotic chromosome synapsis, localizes to axis-associated chromatin in Arabidopsis and Brassica.

10. The pam1 gene is required for meiotic bouquet formation and efficient homologous synapsis in maize (Zea mays L.).

1. Nonlinear structured-illumination microscopy with a photoswitchable protein reveals cellular structures at 50-nm resolution.

2. New technologies for 21st century plant science.

3. Time-lapse two-color 3D imaging of live cells with doubled resolution using structured illumination.

4. Super-resolution 3D microscopy of live whole cells using structured illumination.

Review 5. Optical sectioning microscopy with planar or structured illumination.

6. Super-resolution imaging reveals the internal architecture of nano-sized syntaxin clusters.

Review 7. Advances in high-resolution imaging--techniques for three-dimensional imaging of cellular structures.

8. Dendritic cell podosomes are protrusive and invade the extracellular matrix using metalloproteinase MMP-14.

9. Dopamine Secretion Is Mediated by Sparse Active Zone-like Release Sites.

10. Artifact-free whole-slide imaging with structured illumination microscopy and Bayesian image reconstruction.