Real time quantitative amplification detection on a microarray: towards high multiplex quantitative PCR.

A. Pierik; M Moamfa; M. van Zelst; D. Clout; H. Stapert; Johan Frederik Dijksman; D. Broer; R. Wimberger-Friedl

doi:10.1039/c2lc20740k

Real time quantitative amplification detection on a microarray: towards high multiplex quantitative PCR.

A. Pierik, M Moamfa, M. van Zelst, D. Clout, H. Stapert, Johan Frederik Dijksman, D. Broer, R. Wimberger-Friedl

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Abstract

Quantitative real-time polymerase chain reaction (qrtPCR) is widely used as a research and diagnostic tool. Notwithstanding its many powerful features, the method is limited in the degree of multiplexing to about 6 due to spectral overlap of the available fluorophores. A new method is presented that allows quantitative amplification detection at higher multiplexing by the integration of amplification in solution and monitoring via hybridization to a microarray in real-time. This method does not require any manipulation of the PCR product and runs in a single closed chamber. Employing labeled primers, one of the main challenges is to measure surface signals against a high fluorescence background from solution. A compact, confocal scanner is employed, based on miniaturized optics from DVD technology and combined with a flat thermocycler for simultaneous scanning and heating. The feasibility of this method is demonstrated in singleplex with an analytical sensitivity comparable to routine qrtPCR.

Original language	English
Pages (from-to)	1897-1902
Number of pages	6
Journal	Lab on a chip
Volume	12
DOIs	https://doi.org/10.1039/c2lc20740k
Publication status	Published - 2012

Keywords

METIS-293127
IR-84987

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10.1039/c2lc20740k

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title = "Real time quantitative amplification detection on a microarray: towards high multiplex quantitative PCR.",

abstract = "Quantitative real-time polymerase chain reaction (qrtPCR) is widely used as a research and diagnostic tool. Notwithstanding its many powerful features, the method is limited in the degree of multiplexing to about 6 due to spectral overlap of the available fluorophores. A new method is presented that allows quantitative amplification detection at higher multiplexing by the integration of amplification in solution and monitoring via hybridization to a microarray in real-time. This method does not require any manipulation of the PCR product and runs in a single closed chamber. Employing labeled primers, one of the main challenges is to measure surface signals against a high fluorescence background from solution. A compact, confocal scanner is employed, based on miniaturized optics from DVD technology and combined with a flat thermocycler for simultaneous scanning and heating. The feasibility of this method is demonstrated in singleplex with an analytical sensitivity comparable to routine qrtPCR.",

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year = "2012",

doi = "10.1039/c2lc20740k",

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T1 - Real time quantitative amplification detection on a microarray: towards high multiplex quantitative PCR.

AU - Pierik, A.

AU - Moamfa, M

AU - van Zelst, M.

AU - Clout, D.

AU - Stapert, H.

AU - Dijksman, Johan Frederik

AU - Broer, D.

AU - Wimberger-Friedl, R.

PY - 2012

Y1 - 2012

N2 - Quantitative real-time polymerase chain reaction (qrtPCR) is widely used as a research and diagnostic tool. Notwithstanding its many powerful features, the method is limited in the degree of multiplexing to about 6 due to spectral overlap of the available fluorophores. A new method is presented that allows quantitative amplification detection at higher multiplexing by the integration of amplification in solution and monitoring via hybridization to a microarray in real-time. This method does not require any manipulation of the PCR product and runs in a single closed chamber. Employing labeled primers, one of the main challenges is to measure surface signals against a high fluorescence background from solution. A compact, confocal scanner is employed, based on miniaturized optics from DVD technology and combined with a flat thermocycler for simultaneous scanning and heating. The feasibility of this method is demonstrated in singleplex with an analytical sensitivity comparable to routine qrtPCR.

AB - Quantitative real-time polymerase chain reaction (qrtPCR) is widely used as a research and diagnostic tool. Notwithstanding its many powerful features, the method is limited in the degree of multiplexing to about 6 due to spectral overlap of the available fluorophores. A new method is presented that allows quantitative amplification detection at higher multiplexing by the integration of amplification in solution and monitoring via hybridization to a microarray in real-time. This method does not require any manipulation of the PCR product and runs in a single closed chamber. Employing labeled primers, one of the main challenges is to measure surface signals against a high fluorescence background from solution. A compact, confocal scanner is employed, based on miniaturized optics from DVD technology and combined with a flat thermocycler for simultaneous scanning and heating. The feasibility of this method is demonstrated in singleplex with an analytical sensitivity comparable to routine qrtPCR.

KW - METIS-293127

KW - IR-84987

U2 - 10.1039/c2lc20740k

DO - 10.1039/c2lc20740k

M3 - Article

SN - 1473-0197

VL - 12

SP - 1897

EP - 1902

JO - Lab on a chip

JF - Lab on a chip

ER -

Real time quantitative amplification detection on a microarray: towards high multiplex quantitative PCR.

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Keywords

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