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Literature DB >> 19669529

Axial resolution enhancement by 4Pi confocal fluorescence microscopy with two-photon excitation.

Sylvia Glaschick¹, Carlheinz Röcker, Karen Deuschle, Jörg Wiedenmann, Franz Oswald, Volker Mailänder, G Ulrich Nienhaus.

Abstract

Confocal fluorescence microscopy and two-photon microscopy have become important techniques for the three-dimensional imaging of intact cells. Their lateral resolution is about 200-300 nm for visible light, whereas their axial resolution is significantly worse. By superimposing the spherical wave fronts from two opposing objective lenses in a coherent fashion in 4Pi microscopy, the axial resolution is greatly improved to approximately 100 nm. In combination with specific tagging of proteins or other cellular structures, 4Pi microscopy enables a multitude of molecular interactions in cell biology to be studied. Here, we discuss the choice of appropriate fluorescent tags for dual-color 4Pi microscopy and present applications of this technique in cellular biophysics. We employ two-color fluorescence detection of actin and tubulin networks stained with fluorescent organic dyes; mitochondrial networks are imaged using the photoactivatable fluorescent protein EosFP. A further example concerns the interaction of nanoparticles with mammalian cells.

Entities: Species

Year: 2008 PMID： 19669529 PMCID： PMC2565758 DOI： 10.1007/s10867-008-9084-1

Source DB: PubMed Journal: J Biol Phys ISSN： 0092-0606 Impact factor: 1.365

38 in total

1. Voxx: a PC-based, near real-time volume rendering system for biological microscopy.

Authors: Jeffrey L Clendenon; Carrie L Phillips; Ruben M Sandoval; Shiaofen Fang; Kenneth W Dunn
Journal: Am J Physiol Cell Physiol Date: 2002-01 Impact factor: 4.249

2. Dual-color 4Pi-confocal microscopy with 3D-resolution in the 100 nm range.

Authors: H Kano; S Jakobs; M Nagorni; S W Hell
Journal: Ultramicroscopy Date: 2001-02 Impact factor: 2.689

3. A photoactivatable GFP for selective photolabeling of proteins and cells.

Authors: George H Patterson; Jennifer Lippincott-Schwartz
Journal: Science Date: 2002-09-13 Impact factor: 47.728

4. 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

5. An optical marker based on the UV-induced green-to-red photoconversion of a fluorescent protein.

Authors: Ryoko Ando; Hiroshi Hama; Miki Yamamoto-Hino; Hideaki Mizuno; Atsushi Miyawaki
Journal: Proc Natl Acad Sci U S A Date: 2002-09-23 Impact factor: 11.205

Review 6. Live-cell imaging with EosFP and other photoactivatable marker proteins of the GFP family.

Authors: Jörg Wiedenmann; G Ulrich Nienhaus
Journal: Expert Rev Proteomics Date: 2006-06 Impact factor: 3.940

7. Two-photon excitation and photoconversion of EosFP in dual-color 4Pi confocal microscopy.

Authors: Sergey Ivanchenko; Sylvia Glaschick; Carlheinz Röcker; Franz Oswald; Jörg Wiedenmann; G Ulrich Nienhaus
Journal: Biophys J Date: 2007-03-23 Impact factor: 4.033

Review 8. Advances in fluorescent protein technology.

Authors: Nathan C Shaner; George H Patterson; Michael W Davidson
Journal: J Cell Sci Date: 2007-12-15 Impact factor: 5.285

9. Two-photon fluorescence absorption and emission spectra of dyes relevant for cell imaging.

Authors: F Bestvater; E Spiess; G Stobrawa; M Hacker; T Feurer; T Porwol; U Berchner-Pfannschmidt; C Wotzlaw; H Acker
Journal: J Microsc Date: 2002-11 Impact factor: 1.758

10. Identification of GFP-like proteins in nonbioluminescent, azooxanthellate anthozoa opens new perspectives for bioprospecting.

Authors: Jörg Wiedenmann; Sergey Ivanchenko; Franz Oswald; G Ulrich Nienhaus
Journal: Mar Biotechnol (NY) Date: 2004-05-13 Impact factor: 3.619

5 in total

Axial resolution enhancement by 4Pi confocal fluorescence microscopy with two-photon excitation.

1. Voxx: a PC-based, near real-time volume rendering system for biological microscopy.

2. Dual-color 4Pi-confocal microscopy with 3D-resolution in the 100 nm range.

3. A photoactivatable GFP for selective photolabeling of proteins and cells.

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

5. An optical marker based on the UV-induced green-to-red photoconversion of a fluorescent protein.

Review 6. Live-cell imaging with EosFP and other photoactivatable marker proteins of the GFP family.

7. Two-photon excitation and photoconversion of EosFP in dual-color 4Pi confocal microscopy.

Review 8. Advances in fluorescent protein technology.

9. Two-photon fluorescence absorption and emission spectra of dyes relevant for cell imaging.

10. Identification of GFP-like proteins in nonbioluminescent, azooxanthellate anthozoa opens new perspectives for bioprospecting.

Review 1. Optical imaging of nanoscale cellular structures.

2. Axial resolution improvement of two-photon microscopy by multi-frame reconstruction and adaptive optics.

3. A trimethoprim-based chemical tag for live cell two-photon imaging.

4. 4Pi-RESOLFT nanoscopy.

Review 5. Biomedical Applications for Gold Nanoclusters: Recent Developments and Future Perspectives.