Dynamic imaging of single biomolecular interaction using flow control and TIRFM

T. Arakawa; T. Sameshima; Y. Sato; Y. Sumiyoshi; T. Ueno; Y. Shirasaki; T. Funatsu; S. Shoji

Dynamic imaging of single biomolecular interaction using flow control and TIRFM

T. Arakawa, T. Sameshima, Y. Sato, Y. Sumiyoshi, T. Ueno, Y. Shirasaki, T. Funatsu, S. Shoji

基幹理工学部

研究成果: Paper › 査読

抄録

A rapid multi-reagents switching microvalve system integrated with a total internal reflection fluorescence microscopy (TIRFM) was developed for real time imaging of a single protein behavior. The binding and dissociation process between a chaperonin GroEL and cochaperonin GroES was observed in this TIRFM microfluidic system. For single molecular imaging in this system, biotinylated GroEL (D490C) was immobilized to the glass microchannel surface through streptavidin and biotinylated BSA. A solution including 1 nM IC5-GroES was introduced for 100 ms into the observation area and then washed out with 2 mM ATP buffer solution. Fluorescence spots of IC5-GroES appeared after rapid solution switching, and disappeared several seconds later. As a result, we succeeded in detecting fluorescence signal from single molecules in TIRFM microfluidic system.

本文言語	English
ページ	296-298
ページ数	3
出版ステータス	Published - 2008 1月 1
イベント	12th International Conference on Miniaturized Systems for Chemistry and Life Sciences, MicroTAS 2008 - San Diego, CA, United States 継続期間: 2008 10月 12 → 2008 10月 16

Conference

Conference	12th International Conference on Miniaturized Systems for Chemistry and Life Sciences, MicroTAS 2008
国/地域	United States
City	San Diego, CA
Period	08/10/12 → 08/10/16

ASJC Scopus subject areas

化学工学（その他）
バイオエンジニアリング

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引用スタイル

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title = "Dynamic imaging of single biomolecular interaction using flow control and TIRFM",

abstract = "A rapid multi-reagents switching microvalve system integrated with a total internal reflection fluorescence microscopy (TIRFM) was developed for real time imaging of a single protein behavior. The binding and dissociation process between a chaperonin GroEL and cochaperonin GroES was observed in this TIRFM microfluidic system. For single molecular imaging in this system, biotinylated GroEL (D490C) was immobilized to the glass microchannel surface through streptavidin and biotinylated BSA. A solution including 1 nM IC5-GroES was introduced for 100 ms into the observation area and then washed out with 2 mM ATP buffer solution. Fluorescence spots of IC5-GroES appeared after rapid solution switching, and disappeared several seconds later. As a result, we succeeded in detecting fluorescence signal from single molecules in TIRFM microfluidic system.",

keywords = "Microfluidic device, Single biomolecular imaging, TIRFM",

author = "T. Arakawa and T. Sameshima and Y. Sato and Y. Sumiyoshi and T. Ueno and Y. Shirasaki and T. Funatsu and S. Shoji",

year = "2008",

month = jan,

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language = "English",

pages = "296--298",

note = "12th International Conference on Miniaturized Systems for Chemistry and Life Sciences, MicroTAS 2008 ; Conference date: 12-10-2008 Through 16-10-2008",

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T1 - Dynamic imaging of single biomolecular interaction using flow control and TIRFM

AU - Arakawa, T.

AU - Sameshima, T.

AU - Sato, Y.

AU - Sumiyoshi, Y.

AU - Ueno, T.

AU - Shirasaki, Y.

AU - Funatsu, T.

AU - Shoji, S.

PY - 2008/1/1

Y1 - 2008/1/1

N2 - A rapid multi-reagents switching microvalve system integrated with a total internal reflection fluorescence microscopy (TIRFM) was developed for real time imaging of a single protein behavior. The binding and dissociation process between a chaperonin GroEL and cochaperonin GroES was observed in this TIRFM microfluidic system. For single molecular imaging in this system, biotinylated GroEL (D490C) was immobilized to the glass microchannel surface through streptavidin and biotinylated BSA. A solution including 1 nM IC5-GroES was introduced for 100 ms into the observation area and then washed out with 2 mM ATP buffer solution. Fluorescence spots of IC5-GroES appeared after rapid solution switching, and disappeared several seconds later. As a result, we succeeded in detecting fluorescence signal from single molecules in TIRFM microfluidic system.

AB - A rapid multi-reagents switching microvalve system integrated with a total internal reflection fluorescence microscopy (TIRFM) was developed for real time imaging of a single protein behavior. The binding and dissociation process between a chaperonin GroEL and cochaperonin GroES was observed in this TIRFM microfluidic system. For single molecular imaging in this system, biotinylated GroEL (D490C) was immobilized to the glass microchannel surface through streptavidin and biotinylated BSA. A solution including 1 nM IC5-GroES was introduced for 100 ms into the observation area and then washed out with 2 mM ATP buffer solution. Fluorescence spots of IC5-GroES appeared after rapid solution switching, and disappeared several seconds later. As a result, we succeeded in detecting fluorescence signal from single molecules in TIRFM microfluidic system.

KW - Microfluidic device

KW - Single biomolecular imaging

KW - TIRFM

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T2 - 12th International Conference on Miniaturized Systems for Chemistry and Life Sciences, MicroTAS 2008

Y2 - 12 October 2008 through 16 October 2008

ER -

Dynamic imaging of single biomolecular interaction using flow control and TIRFM

抄録

Conference

ASJC Scopus subject areas

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