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Literature DB >> 16299478

Deep tissue two-photon microscopy.

Abstract

With few exceptions biological tissues strongly scatter light, making high-resolution deep imaging impossible for traditional-including confocal-fluorescence microscopy. Nonlinear optical microscopy, in particular two photon-excited fluorescence microscopy, has overcome this limitation, providing large depth penetration mainly because even multiply scattered signal photons can be assigned to their origin as the result of localized nonlinear signal generation. Two-photon microscopy thus allows cellular imaging several hundred microns deep in various organs of living animals. Here we review fundamental concepts of nonlinear microscopy and discuss conditions relevant for achieving large imaging depths in intact tissue.

Mesh：

Substances：
Fluorescent Dyes

Year: 2005 PMID： 16299478 DOI： 10.1038/nmeth818

Source DB: PubMed Journal: Nat Methods ISSN： 1548-7091 Impact factor: 28.547

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Cited

940 in total

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Deep tissue two-photon microscopy.

1. SCALPEL: EXTRACTING NEURONS FROM CALCIUM IMAGING DATA.

2. Wide field intravital imaging by two-photon-excitation digital-scanned light-sheet microscopy (2p-DSLM) with a high-pulse energy laser.

3. An open source, wireless capable miniature microscope system.

4. Murine Lymphocyte Labeling by 64Cu-Antibody Receptor Targeting for In Vivo Cell Trafficking by PET/CT.

5. Label-free molecular imaging of atherosclerotic lesions using multimodal nonlinear optical microscopy.

6. Two-photon autofluorescence dynamics imaging reveals sensitivity of intracellular NADH concentration and conformation to cell physiology at the single-cell level.

7. Glycinergic interneurons are functionally integrated into the inspiratory network of mouse medullary slices.

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