A new technique for multiparameter imaging microscopy: Use of long decay time photoluminescent labels enables multiple color immunocytochemistry with low channel-to-channel crosstalk

In this report, we describe luminescence imaging microscopy using five different photoluminescent dyes in a single specimen. We combined the long decay time luminophores, europium(III) chelate, terbium(III) chelate, palladium(II) coproporphyrin, and platinum(II) coproporphyrin, with a green nuclear...

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Bibliographic Details
Published in:Microscopy research and technique 2003-12, Vol.62 (5), p.396-407
Main Authors: Soini, Aleksi E., Kuusisto, Ari, Meltola, Niko J., Soini, Erkki, Seveus, Lahja
Format: Article
Language:English
Subjects:
CD3
Fluorescent Dyes - chemistry
Histocytological Preparation Techniques - methods
HNL
Humans
Immunohistochemistry - methods
lanthanide chelates
Leukocytes - cytology
Luminescent Measurements
metalloporphyrins
Microscopy, Fluorescence - methods
MPO
peripheral blood leukocytes
phosphorescence
Specimen Handling - methods
Time Factors
time-resolved fluorescence
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Summary:In this report, we describe luminescence imaging microscopy using five different photoluminescent dyes in a single specimen. We combined the long decay time luminophores, europium(III) chelate, terbium(III) chelate, palladium(II) coproporphyrin, and platinum(II) coproporphyrin, with a green nuclear stain, Syto 25™, that emits conventional fast decaying fluorescence. The luminescence emissions from the five different luminophores were separated from each other by the differences in spectra and decay times using time‐resolved detection. Applicability of this dye‐combination for multiparameter analysis of a biological object was verified in a mixed population of peripheral blood leukocytes. Leukocyte cytocentrifugates were incubated in one step with a cocktail of luminophore‐conjugated antibodies recognizing neutrophil‐ and lymphocyte‐specific markers, followed by rapid staining with a mixture of nuclear stain and Pt‐porphyrin as an eosinophil stain. The results show that multiple luminescent dyes with long decay time can be used together, and in combination with a conventional fluorophore. The separation of the signals of the long decay time labels was distinctive and enabled reliable identification of different leukocyte types, as well as an automated cell count. The long decay time luminophores together with time‐resolved luminescence imaging microscopy (TR‐LIM) provide a unique tool for studies of simultaneous expression of multiple antigens at the level of a single cell. In comparison with other multiparameter imaging techniques, the described technique offers increased accuracy of results, simplification of preparation procedure, and dramatic shortening of the total processing time. To our knowledge, this is the first time that simultaneous fivefold labeling/staining and analysis in a single specimen has been performed in the field of immunocytochemistry. Microsc. Res. Tech. 62:396–407, 2003. © 2003 Wiley‐Liss, Inc.
ISSN:1059-910X
1097-0029
DOI:10.1002/jemt.10389