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Application of FLIM-FIDSAM for the in vivo analysis of hormone competence of different cell types
Authors:Kirstin Elgass  Katharina Caesar  Dierk Wanke  Klaus Harter  Alfred J Meixner  Frank Schleifenbaum
Institution:1. Institute of Physical and Theoretical Chemistry, University of Tübingen, Auf der Morgenstelle 8, 72076, Tübingen, Germany
2. Center for Plant Molecular Biology, Department of Plant Physiology, University of Tübingen, Auf der Morgenstelle 1, 72076, Tübingen, Germany
Abstract:Background fluorescence derived from subcellular compartments is a major drawback in high-resolution live imaging, especially of plant cells. A novel technique for contrast enhancement of fluorescence images of living cells expressing fluorescent fusion proteins termed fluorescence intensity decay shape analysis microscopy (FIDSAM) has been recently published and is applied here to plant cells expressing wild-type levels of a low-abundant membrane protein (BRI1-EGFP), demonstrating the applicability of FIDSAM to samples exhibiting about 80% autofluorescence. Furthermore, the combination of FIDSAM and fluorescence lifetime imaging microscopy enables the simultaneous determination and quantification of different ligand-specific responses in living cells with high spatial and temporal resolution even in samples with high autofluorescence background. Correlation of different responses can be used to determine the hormone ligand competence of different cell types as demonstrated here in BRI1-EGFP-expressing root and hypocotyl cells.
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