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Literature DB >> 24511385

Saturated excitation of fluorescent proteins for subdiffraction-limited imaging of living cells in three dimensions.

Masahito Yamanaka¹, Kenta Saito², Nicholas I Smith³, Satoshi Kawata¹, Takeharu Nagai², Katsumasa Fujita¹.

Abstract

We report, for the first time, the saturated excitation (SAX) of fluorescent proteins for subdiffraction-limited imaging of living cells in three-dimensions. To achieve saturation, a bright yellow and green fluorescent protein (Venus and EGFP) that exhibits a strong nonlinear fluorescence response to the high excitation intensity at the laser focus is used. Harmonic demodulation of the fluorescence signal produced by a modulated excitation light extracts the nonlinear fluorescence signals. After constructing the image from the nonlinear components, we obtain fluorescence images of living cells with spatial resolution beyond the diffraction limit. We also applied linear deconvolution to SAX microscopy and found it effective in further enhancing the contrast of small intracellular structures in the SAX image, confirming the expansion of the optical transfer function in SAX microscopy.

Keywords: confocal microscopy; fluorescence microscopy; high resolution; live-cell imaging; saturated excitation

Year: 2013 PMID： 24511385 PMCID： PMC3915824 DOI： 10.1098/rsfs.2013.0007

Source DB: PubMed Journal: Interface Focus ISSN： 2042-8898 Impact factor: 3.906

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5. Macromolecular-scale resolution in biological fluorescence microscopy.

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6. Video-rate far-field optical nanoscopy dissects synaptic vesicle movement.

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7. Using variable pupil filters to optimize the resolution in multiphoton and saturable fluorescence confocal microscopy.

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2. Thermal illumination limits in 3D Raman microscopy: A comparison of different sample illumination strategies to obtain maximum imaging speed.

Authors: Walter Hauswald; Ronny Förster; Jürgen Popp; Rainer Heintzmann
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2 in total

Saturated excitation of fluorescent proteins for subdiffraction-limited imaging of living cells in three dimensions.

1. Saturated patterned excitation microscopy with two-dimensional excitation patterns.

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

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

4. Live-cell 3D super-resolution imaging in thick biological samples.

5. Macromolecular-scale resolution in biological fluorescence microscopy.

6. Video-rate far-field optical nanoscopy dissects synaptic vesicle movement.

7. Using variable pupil filters to optimize the resolution in multiphoton and saturable fluorescence confocal microscopy.

8. Super-resolution imaging with small organic fluorophores.

9. Optical saturation as a versatile tool to enhance resolution in confocal microscopy.

10. STED nanoscopy of actin dynamics in synapses deep inside living brain slices.

1. Improved two-photon imaging of living neurons in brain tissue through temporal gating.

2. Thermal illumination limits in 3D Raman microscopy: A comparison of different sample illumination strategies to obtain maximum imaging speed.