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Multiexcitation Fluorogenic Labeling of Surface Intracellularand Total Protein Pools in Living Cells

机译:表面细胞内表面的多激发荧光标记和活细胞中的总蛋白池

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摘要

Malachite green (MG) is a fluorogenic dye that shows fluorescence enhancement upon binding to its engineered cognate protein, a fluorogen activating protein (FAP). Energy transfer donors such as cyanine and rhodamine dyes have been conjugated with MG to modify the spectral properties of the fluorescent complexes, where the donor dyes transfer energy through Förster resonance energy transfer to the MG complex resulting in binding-conditional fluorescence emission in the far-red region. In this article, we use a violet-excitable dye as a donor to sensitize the far-red emission of the MG-FAP complex. Two blue emitting fluorescent coumarin dyes were coupled to MG and evaluated for energy transfer to the MG-FAP complex via its secondary excitation band. 6,8-Difluoro-7-hydroxycoumarin-3-carboxylic acid (Pacific blue, PB) showed the most efficient energy transfer and maximum brightness in the far-red region upon violet (405 nm) excitation. These blue-red (BluR) tandem dyes are spectrally varied from other tandem dyes and are able to produce fluorescence images of the MG-FAP complex witha large Stokes shift (>250 nm). These dyes are cell-permeable andare used to label intracellular proteins. Used together with a cell-impermeablehexa-Cy3-MG (HCM) dye that labels extracellular proteins, we are ableto visualize extracellular, intracellular, and total pools of cellularprotein using one fluorogenic tag that combines with distinct dyesto effect different spectral characteristics.
机译:孔雀石绿(MG)是一种发荧光的染料,结合到其工程化同源蛋白即荧光激活蛋白(FAP)后,荧光增强。能量转移供体(例如花青和罗丹明染料)已与MG结合,以改变荧光配合物的光谱特性,其中供体染料通过Förster共振能量转移将能量转移至MG配合物,从而导致远处的结合条件荧光发射红色区域。在本文中,我们使用紫罗兰色可激发染料作为供体来敏化MG-FAP复合物的远红外发射。将两种发蓝光的荧光香豆素染料与MG偶联,并通过其次级激发带评估向MG-FAP复合物的能量转移。 6,8-二氟-7-羟基香豆素-3-羧酸(太平洋蓝,PB)在紫光(405 nm)激发下,在远红区域显示出最有效的能量传递和最大亮度。这些蓝红色(BluR)串联染料在光谱上不同于其他串联染料,并能够产生MG-FAP配合物的荧光图像较大的斯托克斯位移(> 250 nm)。这些染料具有细胞渗透性和用于标记细胞内蛋白。与不可渗透细胞一起使用六-Cy3-MG(HCM)染料标记细胞外蛋白,我们能够可视化细胞外,细胞内和总细胞池一种荧光标记结合独特的染料合成蛋白质影响不同的光谱特性。

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