Literature DB >> 17557785

The power of single and multibeam two-photon microscopy for high-resolution and high-speed deep tissue and intravital imaging.

Raluca Niesner1, Volker Andresen, Jens Neumann, Heinrich Spiecker, Matthias Gunzer.   

Abstract

Two-photon microscopy is indispensable for deep tissue and intravital imaging. However, current technology based on single-beam point scanning has reached sensitivity and speed limits because higher performance requires higher laser power leading to sample degradation. We utilize a multifocal scanhead splitting a laser beam into a line of 64 foci, allowing sample illumination in real time at full laser power. This technology requires charge-coupled device field detection in contrast to conventional detection by photomultipliers. A comparison of the optical performance of both setups shows functional equivalence in every measurable parameter down to penetration depths of 200 microm, where most actual experiments are executed. The advantage of photomultiplier detection materializes at imaging depths >300 microm because of their better signal/noise ratio, whereas only charge-coupled devices allow real-time detection of rapid processes (here blood flow). We also find that the point-spread function of both devices strongly depends on tissue constitution and penetration depth. However, employment of a depth-corrected point-spread function allows three-dimensional deconvolution of deep-tissue data up to an image quality resembling surface detection.

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Year:  2007        PMID: 17557785      PMCID: PMC1965440          DOI: 10.1529/biophysj.106.102459

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


  25 in total

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4.  Improvement of transcutaneous fluorescent images with a depth-dependent point-spread function.

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6.  Adaptive wavefront correction in two-photon microscopy using coherence-gated wavefront sensing.

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Journal:  Proc Natl Acad Sci U S A       Date:  2006-11-06       Impact factor: 11.205

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8.  Two-photon laser scanning fluorescence microscopy.

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10.  Functional fluorescent Ca2+ indicator proteins in transgenic mice under TET control.

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Journal:  PLoS Biol       Date:  2004-06-15       Impact factor: 8.029

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  39 in total

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Review 3.  3D and 4D imaging of immune cells in vitro and in vivo.

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4.  Encoded multisite two-photon microscopy.

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5.  Two-photon 3D FIONA of individual quantum dots in an aqueous environment.

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6.  Expanding two-photon intravital microscopy to the infrared by means of optical parametric oscillator.

Authors:  Josephine Herz; Volker Siffrin; Anja E Hauser; Alexander U Brandt; Tina Leuenberger; Helena Radbruch; Frauke Zipp; Raluca A Niesner
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Review 7.  Nonlinear absorption microscopy.

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8.  Intravital confocal and two-photon imaging of dual-color cells and extracellular matrix mimics.

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

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Review 10.  Cardiovascular imaging using two-photon microscopy.

Authors:  John A Scherschel; Michael Rubart
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