Modulation-frequency encoded multi-color fluorescent DNA analysis in an optofluidic chip

We introduce a principle of parallel optical processing to an optofluidic lab-on-a-chip. During electrophoretic separation, the ultra-low limit of detection achieved with our set-up allows us to record fluorescence from covalently end-labeled DNA molecules. Different sets of exclusively color-labele...

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Veröffentlicht in:Lab on a chip 2011-02, Vol.11 (4), p.679-683
Hauptverfasser: Dongre, Chaitanya, van Weerd, Jasper, Besselink, Geert A. J, Vazquez, Rebeca Martinez, Osellame, Roberto, Cerullo, Giulio, van Weeghel, Rob, van den Vlekkert, Hans H, Hoekstra, Hugo J. W. M, Pollnau, Markus
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Sprache:eng
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Zusammenfassung:We introduce a principle of parallel optical processing to an optofluidic lab-on-a-chip. During electrophoretic separation, the ultra-low limit of detection achieved with our set-up allows us to record fluorescence from covalently end-labeled DNA molecules. Different sets of exclusively color-labeled DNA fragments-otherwise rendered indistinguishable by spatio-temporal coincidence-are traced back to their origin by modulation-frequency-encoded multi-wavelength laser excitation, fluorescence detection with a single ultrasensitive, albeit color-blind photomultiplier, and Fourier analysis decoding. As a proof of principle, fragments obtained by multiplex ligation-dependent probe amplification from independent human genomic segments, associated with genetic predispositions to breast cancer and anemia, are simultaneously analyzed. We introduce a principle of parallel optical processing to an optofluidic lab-on-a-chip. During electrophoretic separation, the ultra-low limit of detection achieved with our set-up allows us to record fluorescence from covalently end-labeled DNA molecules.
ISSN:1473-0197
1473-0189
DOI:10.1039/c0lc00449a