Literature DB >> 1326429

Time-resolved fluorescence imaging of europium chelate label in immunohistochemistry and in situ hybridization.

L Seveus1, M Väisälä, S Syrjänen, M Sandberg, A Kuusisto, R Harju, J Salo, I Hemmilä, H Kojola, E Soini.   

Abstract

Fluorescent lanthanide chelates with long decay times allow the suppression of the fast decaying autofluorescence in biological specimens. This property makes lanthanide chelates attractive as labels for fluorescence microscopy. As a consequence of the suppression of the background fluorescence the sensitivity can be increased. We modified a standard epifluorescence microscope for time-resolved fluorescence imaging by adding a pulsed light source and a chopper in the narrow aperture plane. A cooled CCD-camera was used for detection and the images were digitally processed. A fluorescent europium chelate was conjugated to antisera and to streptavidin. These conjugates were used for the localization of tumor associated antigen C242 in the malignant mucosa of human colon, for the localization of type II collagen mRNA in developing human cartilaginary growth plates, and for the detection of HPV type specific gene sequences in the squamous epithelium of human cervix. The specific slowly decaying fluorescence of the europium label could be effectively separated from the fast decaying background fluorescence. It was possible to use the europium label at the cell and tissue level and the autofluorescence was effectively suppressed in in situ hybridization and immunohistochemical reactions in both frozen and formaldehyde-fixed, wax-embedded specimens.

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Year:  1992        PMID: 1326429     DOI: 10.1002/cyto.990130402

Source DB:  PubMed          Journal:  Cytometry        ISSN: 0196-4763


  18 in total

1.  Two color RNA intercalating probe for cell imaging applications.

Authors:  Nathan Stevens; Naphtali O'Connor; Harshad Vishwasrao; Diana Samaroo; Eric R Kandel; Daniel L Akins; Charles M Drain; Nicholas J Turro
Journal:  J Am Chem Soc       Date:  2008-05-20       Impact factor: 15.419

Review 2.  Cytochemical detection systems for in situ hybridization, and the combination with immunocytochemistry, 'who is still afraid of red, green and blue?'.

Authors:  E J Speel; F C Ramaekers; A H Hopman
Journal:  Histochem J       Date:  1995-11

3.  Synthesis and evaluation of phosphorescent oligonucleotide probes for hybridisation assays.

Authors:  Paul J O'Sullivan; Martina Burke; Aleksi E Soini; Dmitri B Papkovsky
Journal:  Nucleic Acids Res       Date:  2002-11-01       Impact factor: 16.971

4.  Temporally and spectrally resolved imaging microscopy of lanthanide chelates.

Authors:  G Vereb; E Jares-Erijman; P R Selvin; T M Jovin
Journal:  Biophys J       Date:  1998-05       Impact factor: 4.033

Review 5.  Lanthanide-Based Optical Probes of Biological Systems.

Authors:  Ukrae Cho; James K Chen
Journal:  Cell Chem Biol       Date:  2020-07-30       Impact factor: 8.116

6.  High-sensitivity detection of cardiac troponin I with UV LED excitation for use in point-of-care immunoassay.

Authors:  Olga Rodenko; Susann Eriksson; Peter Tidemand-Lichtenberg; Carl Peder Troldborg; Henrik Fodgaard; Sylvana van Os; Christian Pedersen
Journal:  Biomed Opt Express       Date:  2017-07-20       Impact factor: 3.732

7.  Time-resolved delayed luminescence image microscopy using an europium ion chelate complex.

Authors:  G Marriott; M Heidecker; E P Diamandis; Y Yan-Marriott
Journal:  Biophys J       Date:  1994-09       Impact factor: 4.033

8.  Multicolour preparations for in situ hybridization using precipitating enzyme cytochemistry in combination with reflection contrast microscopy.

Authors:  E J Speel; M Kamps; J Bonnet; F C Ramaekers; A H Hopman
Journal:  Histochemistry       Date:  1993-11

9.  Time Gated Luminescence Imaging of Immunolabeled Human Tissues.

Authors:  Ting Chen; Rui Hong; Darren Magda; Christopher Bieniarz; Larry Morrison; Lawrence W Miller
Journal:  Anal Chem       Date:  2017-11-15       Impact factor: 6.986

10.  Reflectance enzyme histochemistry (REH): visualization of cerium-based and DAB primary reaction products of phosphatases and oxidases in cryostat sections by confocal laser scanning microscopy.

Authors:  K J Halbhuber; C Scheven; G Jirikowski; H Feuerstein; U Ott
Journal:  Histochem Cell Biol       Date:  1996-03       Impact factor: 4.304

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