Quantitative Analysis of Photodamage During Fluorescence Bioimaging: Monitoring of Nitric Oxide Production using DAF-2

DOI 14 References
  • Kuroda Takashi
    Department of Histology, School of Medicine, Iwate Medical University
  • Satoh Yoh-ichi
    Department of Histology, School of Medicine, Iwate Medical University
  • Akutsu-Yamauchi Hitomi
    Department of Histology, School of Medicine, Iwate Medical University
  • Shikanai Yuuki
    Department of Histology, School of Medicine, Iwate Medical University
  • Miyata Setsuya
    Department of Histology, School of Medicine, Iwate Medical University
  • Saino Tomoyuki
    Department of Histology, School of Medicine, Iwate Medical University
  • Russa Denis
    Department of Histology, School of Medicine, Iwate Medical University
  • Habara Yoshiaki
    Laboratory of Physiology, The Graduate School of Veterinary Medicine, Hokkaido University
  • Cui Zon-Jie
    Institute of Cell Biology, Beijing Normal University

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Abstract

Photodamage occurs, to a greater or lesser extent, during fluorescence bioimaging, and various procedures are empirically used to reduce the extent of this damage. However, measuring photodamage is difficult. Nitric oxide (NO), a gaseous messenger, is a free radical, and can be induced by light-exposure. In the present study, NO production was determined by the treatment of cultured cardiomyocytes, hippocampal neurons, dorsal root ganglion cells and serous peritoneal mast cells with 4, 5-diaminofluorescein (DAF-2). During laser irradiation in confocal microscopy, the fluorescence intensity of DAF-2 was increased in many punctuate regions of the cytoplasm as well as the nuclei of the cells examined. After the increase in NO levels, the beating of cardiomyocytes and the exocytosis of mast cells ceased. A stronger laser power caused a more intense peak and a more rapid increase in NO production. NO production in mast cells under various conditions was observed, in an attempt to reduce the extent of photodamage. Intermittent irradiation had no effect on NO production. Anti-oxidants (bovine serum albumin, vitamin E and melatonin), inhibited the peak and delayed the time course for NO production at a weak laser power, but had no effect on the bleaching of Indo-1, a fluorescent calcium indicator. In all bioimaging experiments in which a fluorescence technique is involved, the possibility of photodamage should be considered, and monitoring NO production by DAF-2 continues to be a relatively straightforward method for detecting photodamage.

Journal

  • bioimages

    bioimages 14 9-18, 2006

    Bioimaging Society

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Details 詳細情報について

  • CRID
    1390282679413353984
  • NII Article ID
    10020936919
  • NII Book ID
    AA11084187
  • DOI
    10.11169/bioimages.14.9
  • COI
    1:CAS:528:DC%2BD2sXjsl2qtr4%3D
  • ISSN
    09192719
  • Text Lang
    en
  • Data Source
    • JaLC
    • CiNii Articles
    • KAKEN
  • Abstract License Flag
    Disallowed

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