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      Highly resolved intravital striped-illumination microscopy of germinal centers.

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          Abstract

          Monitoring cellular communication by intravital deep-tissue multi-photon microscopy is the key for understanding the fate of immune cells within thick tissue samples and organs in health and disease. By controlling the scanning pattern in multi-photon microscopy and applying appropriate numerical algorithms, we developed a striped-illumination approach, which enabled us to achieve 3-fold better axial resolution and improved signal-to-noise ratio, i.e. contrast, in more than 100 µm tissue depth within highly scattering tissue of lymphoid organs as compared to standard multi-photon microscopy. The acquisition speed as well as photobleaching and photodamage effects were similar to standard photo-multiplier-based technique, whereas the imaging depth was slightly lower due to the use of field detectors. By using the striped-illumination approach, we are able to observe the dynamics of immune complex deposits on secondary follicular dendritic cells - on the level of a few protein molecules in germinal centers.

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          Author and article information

          Journal
          J Vis Exp
          Journal of visualized experiments : JoVE
          MyJove Corporation
          1940-087X
          1940-087X
          Apr 09 2014
          : 86
          Affiliations
          [1 ] Biophysical Analytics, German Rheumatism Research Center, Leibniz Institute; Microscopy Core Facility, Max-Delbrück Center for Molecular Medicine.
          [2 ] Immunodynamics, German Rheumatism Research Center, Leibniz Institute.
          [3 ] LaVision Biotec GmbH.
          [4 ] Microscopy Core Facility, Max-Delbrück Center for Molecular Medicine.
          [5 ] Immunodynamics, German Rheumatism Research Center, Leibniz Institute; Immunodynamics and Intravital Imaging, Charité - University of Medicine; hauser@drfz.de.
          [6 ] Biophysical Analytics, German Rheumatism Research Center, Leibniz Institute; niesner@drfz.de.
          Article
          10.3791/51135
          4165301
          24748007
          c350a85a-fb8a-4c95-a390-54411961091b
          History

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