A rapid SNAP-tag fluorogenic probe based on an environment-sensitive fluorophore for no-wash live cell imaging

Tao Kai Liu; Pei Ying Hsieh; Yu De Zhuang; Chi Yang Hsia; Chi Ling Huang; Hsiu Ping Lai; Hung Sheung Lin; I. Chia Chen; Hsin-Yun Hsu; Kui Thong Tan

doi:10.1021/cb500502n

A rapid SNAP-tag fluorogenic probe based on an environment-sensitive fluorophore for no-wash live cell imaging

Tao Kai Liu, Pei Ying Hsieh, Yu De Zhuang, Chi Yang Hsia, Chi Ling Huang, Hsiu Ping Lai, Hung Sheung Lin, I. Chia Chen, Hsin-Yun Hsu^*, Kui Thong Tan

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46 引文斯高帕斯（Scopus）

摘要

(Figure Presented). One major limitation of labeling proteins with synthetic fluorophores is the high fluorescence background, which necessitates extensive washing steps to remove unreacted fluorophores. In this paper, we describe a novel fluorogenic probe based on an environment-sensitive fluorophore for labeling with SNAP-tag proteins. The probe exhibits dramatic fluorescence turn-on of 280-fold upon being labeled to SNAP-tag. The major advantages of our fluorogenic probe are the dramatic fluorescence turn-on, ease of synthesis, high selectivity, and rapid labeling with SNAP-tag. No-wash labeling of both intracellular and cell surface proteins was successfully achieved in living cells, and the localization of these proteins was specifically visualized.

原文	English
頁（從 - 到）	2359-2365
頁數	7
期刊	ACS Chemical Biology
卷	9
發行號	10
DOIs	https://doi.org/10.1021/cb500502n
出版狀態	Published - 8 8月 2014

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10.1021/cb500502n

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title = "A rapid SNAP-tag fluorogenic probe based on an environment-sensitive fluorophore for no-wash live cell imaging",

abstract = "(Figure Presented). One major limitation of labeling proteins with synthetic fluorophores is the high fluorescence background, which necessitates extensive washing steps to remove unreacted fluorophores. In this paper, we describe a novel fluorogenic probe based on an environment-sensitive fluorophore for labeling with SNAP-tag proteins. The probe exhibits dramatic fluorescence turn-on of 280-fold upon being labeled to SNAP-tag. The major advantages of our fluorogenic probe are the dramatic fluorescence turn-on, ease of synthesis, high selectivity, and rapid labeling with SNAP-tag. No-wash labeling of both intracellular and cell surface proteins was successfully achieved in living cells, and the localization of these proteins was specifically visualized.",

author = "Liu, {Tao Kai} and Hsieh, {Pei Ying} and Zhuang, {Yu De} and Hsia, {Chi Yang} and Huang, {Chi Ling} and Lai, {Hsiu Ping} and Lin, {Hung Sheung} and Chen, {I. Chia} and Hsin-Yun Hsu and Tan, {Kui Thong}",

year = "2014",

month = aug,

day = "8",

doi = "10.1021/cb500502n",

language = "English",

volume = "9",

pages = "2359--2365",

journal = "ACS Chemical Biology",

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T1 - A rapid SNAP-tag fluorogenic probe based on an environment-sensitive fluorophore for no-wash live cell imaging

AU - Liu, Tao Kai

AU - Hsieh, Pei Ying

AU - Zhuang, Yu De

AU - Hsia, Chi Yang

AU - Huang, Chi Ling

AU - Lai, Hsiu Ping

AU - Lin, Hung Sheung

AU - Chen, I. Chia

AU - Hsu, Hsin-Yun

AU - Tan, Kui Thong

PY - 2014/8/8

Y1 - 2014/8/8

N2 - (Figure Presented). One major limitation of labeling proteins with synthetic fluorophores is the high fluorescence background, which necessitates extensive washing steps to remove unreacted fluorophores. In this paper, we describe a novel fluorogenic probe based on an environment-sensitive fluorophore for labeling with SNAP-tag proteins. The probe exhibits dramatic fluorescence turn-on of 280-fold upon being labeled to SNAP-tag. The major advantages of our fluorogenic probe are the dramatic fluorescence turn-on, ease of synthesis, high selectivity, and rapid labeling with SNAP-tag. No-wash labeling of both intracellular and cell surface proteins was successfully achieved in living cells, and the localization of these proteins was specifically visualized.

AB - (Figure Presented). One major limitation of labeling proteins with synthetic fluorophores is the high fluorescence background, which necessitates extensive washing steps to remove unreacted fluorophores. In this paper, we describe a novel fluorogenic probe based on an environment-sensitive fluorophore for labeling with SNAP-tag proteins. The probe exhibits dramatic fluorescence turn-on of 280-fold upon being labeled to SNAP-tag. The major advantages of our fluorogenic probe are the dramatic fluorescence turn-on, ease of synthesis, high selectivity, and rapid labeling with SNAP-tag. No-wash labeling of both intracellular and cell surface proteins was successfully achieved in living cells, and the localization of these proteins was specifically visualized.

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DO - 10.1021/cb500502n

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SN - 1554-8929

VL - 9

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EP - 2365

JO - ACS Chemical Biology

JF - ACS Chemical Biology

IS - 10

ER -

A rapid SNAP-tag fluorogenic probe based on an environment-sensitive fluorophore for no-wash live cell imaging

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