High-Throughput Nanohole Array Based System To Monitor Multiple Binding Events in Real Time

We have developed an integrated label-free, real-time sensing system that is able to monitor multiple biomolecular binding events based on the changes in the intensity of extraordinary optical transmission (EOT) through nanohole arrays. The core of the system is a sensing chip containing multiple na...

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Veröffentlicht in:	Analytical chemistry (Washington) 2008-04, Vol.80 (7), p.2491-2498
Hauptverfasser:	Ji, Jin, O'Connell, J. Garland, Carter, David J. D, Larson, Dale N
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Sprache:	eng
Schlagworte:	Analytical chemistry Antibodies - immunology Antigens - immunology Binding sites Biochemistry Biosensing Techniques Biosensors Chemistry Electrons Exact sciences and technology General, instrumentation Microarray Analysis - instrumentation Microarray Analysis - methods Nanostructures - chemistry Proteomics Studies Temperature Time Factors
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creator	Ji, Jin O'Connell, J. Garland Carter, David J. D Larson, Dale N
description	We have developed an integrated label-free, real-time sensing system that is able to monitor multiple biomolecular binding events based on the changes in the intensity of extraordinary optical transmission (EOT) through nanohole arrays. The core of the system is a sensing chip containing multiple nanohole arrays embedded within an optically thick gold film, where each array functions as an independent sensor. Each array is a square array containing 10 × 10 nanoholes (150 nm in diameter), occupying a total area of 3.3 μm × 3.3 μm. The integrated system includes a laser light source, a temperature-regulated flow cell encasing the sensing chip, motorized optics, and a charge-coupled detector (CCD) camera. For demonstration purposes, sensing chips containing 25 nanohole arrays were studied for their use in multiplexed detection, although the sensing chip could be easily populated to contain up to 20 164 nanohole arrays within its 0.64 cm2 sensing area. Using this system, we successfully recorded 25 separate binding curves between glutathione S-transferase (GST) and anti-GST simultaneously in real time with good sensitivity. The system responds to binding events in a concentration-dependent manner, showing a sharp linear response to anti-GST at concentrations ranging from 13 to 290 nM. The EOT intensity-based approach also enables the system to monitor multiple bindings simultaneously and continuously, offering a temporal resolution on milliseconds scale that is decided only by the camera speed and exposure time. The small footprint of the sensing arrays combined with the EOT intensity-based approach enables the system to resolve binding events that occurred on nanohole sensing arrays spaced 96 μm apart, with a reasonable prediction of resolving binding events spaced 56 μm apart. This work represents a new direction that implements nanohole arrays and EOT intensity to meet high-throughput, spatial and temporal resolution, and sensitivity requirements in drug discovery and proteomics studies.
doi_str_mv	10.1021/ac7023206
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For demonstration purposes, sensing chips containing 25 nanohole arrays were studied for their use in multiplexed detection, although the sensing chip could be easily populated to contain up to 20 164 nanohole arrays within its 0.64 cm2 sensing area. Using this system, we successfully recorded 25 separate binding curves between glutathione S-transferase (GST) and anti-GST simultaneously in real time with good sensitivity. The system responds to binding events in a concentration-dependent manner, showing a sharp linear response to anti-GST at concentrations ranging from 13 to 290 nM. The EOT intensity-based approach also enables the system to monitor multiple bindings simultaneously and continuously, offering a temporal resolution on milliseconds scale that is decided only by the camera speed and exposure time. The small footprint of the sensing arrays combined with the EOT intensity-based approach enables the system to resolve binding events that occurred on nanohole sensing arrays spaced 96 μm apart, with a reasonable prediction of resolving binding events spaced 56 μm apart. 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The small footprint of the sensing arrays combined with the EOT intensity-based approach enables the system to resolve binding events that occurred on nanohole sensing arrays spaced 96 μm apart, with a reasonable prediction of resolving binding events spaced 56 μm apart. 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Garland</au><au>Carter, David J. D</au><au>Larson, Dale N</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>High-Throughput Nanohole Array Based System To Monitor Multiple Binding Events in Real Time</atitle><jtitle>Analytical chemistry (Washington)</jtitle><addtitle>Anal. Chem</addtitle><date>2008-04-01</date><risdate>2008</risdate><volume>80</volume><issue>7</issue><spage>2491</spage><epage>2498</epage><pages>2491-2498</pages><issn>0003-2700</issn><eissn>1520-6882</eissn><coden>ANCHAM</coden><abstract>We have developed an integrated label-free, real-time sensing system that is able to monitor multiple biomolecular binding events based on the changes in the intensity of extraordinary optical transmission (EOT) through nanohole arrays. The core of the system is a sensing chip containing multiple nanohole arrays embedded within an optically thick gold film, where each array functions as an independent sensor. Each array is a square array containing 10 × 10 nanoholes (150 nm in diameter), occupying a total area of 3.3 μm × 3.3 μm. The integrated system includes a laser light source, a temperature-regulated flow cell encasing the sensing chip, motorized optics, and a charge-coupled detector (CCD) camera. For demonstration purposes, sensing chips containing 25 nanohole arrays were studied for their use in multiplexed detection, although the sensing chip could be easily populated to contain up to 20 164 nanohole arrays within its 0.64 cm2 sensing area. Using this system, we successfully recorded 25 separate binding curves between glutathione S-transferase (GST) and anti-GST simultaneously in real time with good sensitivity. The system responds to binding events in a concentration-dependent manner, showing a sharp linear response to anti-GST at concentrations ranging from 13 to 290 nM. The EOT intensity-based approach also enables the system to monitor multiple bindings simultaneously and continuously, offering a temporal resolution on milliseconds scale that is decided only by the camera speed and exposure time. The small footprint of the sensing arrays combined with the EOT intensity-based approach enables the system to resolve binding events that occurred on nanohole sensing arrays spaced 96 μm apart, with a reasonable prediction of resolving binding events spaced 56 μm apart. This work represents a new direction that implements nanohole arrays and EOT intensity to meet high-throughput, spatial and temporal resolution, and sensitivity requirements in drug discovery and proteomics studies.</abstract><cop>Washington, DC</cop><pub>American Chemical Society</pub><pmid>18307360</pmid><doi>10.1021/ac7023206</doi><tpages>8</tpages></addata></record>
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subjects	Analytical chemistry Antibodies - immunology Antigens - immunology Binding sites Biochemistry Biosensing Techniques Biosensors Chemistry Electrons Exact sciences and technology General, instrumentation Microarray Analysis - instrumentation Microarray Analysis - methods Nanostructures - chemistry Proteomics Studies Temperature Time Factors
title	High-Throughput Nanohole Array Based System To Monitor Multiple Binding Events in Real Time
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