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Literature DB >> 11413041

Lighting up the cell surface with evanescent wave microscopy.

Abstract

Evanescent wave microscopy, also termed total internal reflection fluorescence microscopy (TIR-FM), has shed new light on important cellular processes taking place near the plasma membrane. For example, this technique can enable the direct observation of membrane fusion of synaptic vesicles and the movement of single molecules during signal transduction. There has been a recent surge in the popularity of this technique with the advent of green-fluorescent protein (GFP) as a fluorescent marker and new technical developments. These technical developments and some of the latest applications of TIR-FM are the subject of this review.

Mesh：

Substances：
Fluorescent Dyes

Year: 2001 PMID： 11413041 DOI： 10.1016/s0962-8924(01)02027-x

Source DB: PubMed Journal: Trends Cell Biol ISSN： 0962-8924 Impact factor: 20.808

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Cited

48 in total

1. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts: II. Parameter estimates for individual cells from experiments.

Authors: Ian C Schneider; Jason M Haugh
Journal: Biophys J Date: 2004-01 Impact factor: 4.033

2. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts: I. Uniform stimulation model and bounds on dimensionless groups.

Authors: Jason M Haugh; Ian C Schneider
Journal: Biophys J Date: 2004-01 Impact factor: 4.033

3. Single-molecule investigation of the interference between kinesin, tau and MAP2c.

Authors: Arne Seitz; Hiroaki Kojima; Kazuhiro Oiwa; Eva-Maria Mandelkow; Young-Hwa Song; Eckhard Mandelkow
Journal: EMBO J Date: 2002-09-16 Impact factor: 11.598

4. Imaging the activity and localization of single voltage-gated Ca(2+) channels by total internal reflection fluorescence microscopy.

Authors: Angelo Demuro; Ian Parker
Journal: Biophys J Date: 2004-05 Impact factor: 4.033

5. Synaptic vesicle exocytosis in hippocampal synaptosomes correlates directly with total mitochondrial volume.

Authors: Maxim V Ivannikov; Mutsuyuki Sugimori; Rodolfo R Llinás
Journal: J Mol Neurosci Date: 2012-07-08 Impact factor: 3.444

6. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts, III: influence of cell morphology and morphological Polarity.

Authors: Ian C Schneider; Elizabeth M Parrish; Jason M Haugh
Journal: Biophys J Date: 2005-05-27 Impact factor: 4.033

Lighting up the cell surface with evanescent wave microscopy.

1. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts: II. Parameter estimates for individual cells from experiments.

2. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts: I. Uniform stimulation model and bounds on dimensionless groups.

3. Single-molecule investigation of the interference between kinesin, tau and MAP2c.

4. Imaging the activity and localization of single voltage-gated Ca(2+) channels by total internal reflection fluorescence microscopy.

5. Synaptic vesicle exocytosis in hippocampal synaptosomes correlates directly with total mitochondrial volume.

6. Spatial analysis of 3' phosphoinositide signaling in living fibroblasts, III: influence of cell morphology and morphological Polarity.

7. Initiation of attachment and generation of mature focal adhesions by integrin-containing filopodia in cell spreading.

8. Live-cell imaging of receptors around postsynaptic membranes.

9. Interference reflection microscopy.

Review 10. Endocytic events in TCR signaling: focus on adapters in microclusters.