Fluorescence lifetime endoscopy using TCSPC for the measurement of FRET in live cells

Gilbert O. Fruhwirth, Simon Ameer-Beg, Richard Cook, Timothy Watson, Tony Ng, Frederic Festy

Research output: Contribution to journalArticlepeer-review

48 Citations (Scopus)
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Abstract

Development of remote imaging for diagnostic purposes has progressed dramatically since endoscopy began in the 1960's. The recent advent of a clinically licensed intensity-based fluorescence micro-endoscopic instrument has offered the prospect of real-time cellular resolution imaging. However, interrogating protein-protein interactions deep inside living tissue requires precise fluorescence lifetime measurements to derive the Forster resonance energy transfer between two tagged fluorescent markers. We developed a new instrument combining remote fiber endoscopic cellular-resolution imaging with TCSPC-FLIM technology to interrogate and discriminate mixed fluorochrome labeled beads and expressible GFP/TagRFP tags within live cells. Endoscopic-FLIM (e-FLIM) data was validated by comparison with data acquired via conventional FLIM and e-FLIM was found to be accurate for both bright bead and dim live cell samples. The fiber based micro-endoscope allowed remote imaging of 4 mu m and 10 mu m beads within a thick Matrigel matrix with confident fluorophore discrimination using lifetime information. More importantly, this new technique enabled us to reliably measure protein-protein interactions in live cells embedded in a 3D matrix, as demonstrated by the dimerization of the fluorescent protein-tagged membrane receptor CXCR4. This cell-based application successfully demonstrated the suitability and great potential of this new technique for in vivo pre-clinical biomedical and possibly human clinical applications. (C) 2010 Optical Society of America
Original languageEnglish
Pages (from-to)11148 - 11158
Number of pages11
JournalOPTICS EXPRESS
Volume18
Issue number11
DOIs
Publication statusPublished - 24 May 2010

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