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吖啶橙与增强型绿色荧光蛋白在星形胶质细胞囊泡细胞器中的系统性共定位误差。

Systematic colocalization errors between acridine orange and EGFP in astrocyte vesicular organelles.

作者信息

Nadrigny Fabien, Li Dongdong, Kemnitz Klaus, Ropert Nicole, Koulakoff Annette, Rudolph Stephanie, Vitali Marco, Giaume Christian, Kirchhoff Frank, Oheim Martin

机构信息

INSERM, U603, Paris, France.

出版信息

Biophys J. 2007 Aug 1;93(3):969-80. doi: 10.1529/biophysj.106.102673. Epub 2007 Apr 6.

Abstract

Dual-color imaging of acridine orange (AO) and EGFP fused to a vesicular glutamate transporter or the vesicle-associated membrane proteins 2 or 3 has been used to visualize a supposedly well-defined subpopulation of glutamatergic astrocytic secretory vesicles undergoing regulated exocytosis. However, AO metachromasy results in the concomitant emission of green and red fluorescence from AO-stained tissue. Therefore, the question arises whether AO and EGFP fluorescence can be distinguished reliably. We used evanescent-field imaging with spectral fluorescence detection as well as fluorescence lifetime imaging microscopy to demonstrate that green fluorescent AO monomers inevitably coexist with red fluorescing AO dimers, at the level of single astroglial vesicles. The green monomer emission spectrally overlaps with that of EGFP and produces a false apparent colocalization on dual-color images. On fluorophore abundance maps calculated from spectrally resolved and unmixed single-vesicle spectral image stacks, EGFP is obscured by the strong green monomer fluorescence, precluding the detection of EGFP. Hence, extreme caution is required when deriving quantitative colocalization information from images of dim fluorescing EGFP-tagged organelles colabeled with bright and broadly emitting dyes like AO. We finally introduce FM4-64/EGFP dual-color imaging as a remedy for imaging a distinct population of astroglial fusion-competent secretory vesicles.

摘要

将吖啶橙(AO)与融合了囊泡谷氨酸转运体、囊泡相关膜蛋白2或3的增强型绿色荧光蛋白(EGFP)进行双色成像,已被用于观察一群假定定义明确的谷氨酸能星形胶质细胞分泌囊泡,这些囊泡正在经历受调控的胞吐作用。然而,AO的异染性导致AO染色组织同时发出绿色和红色荧光。因此,是否能可靠地区分AO和EGFP荧光就成了问题。我们使用了具有光谱荧光检测功能的倏逝场成像以及荧光寿命成像显微镜,以证明在单个星形胶质细胞囊泡水平上,绿色荧光的AO单体不可避免地与红色荧光的AO二聚体共存。绿色单体发射光谱与EGFP的光谱重叠,在双色图像上产生了假的明显共定位。在从光谱分辨和非混合的单囊泡光谱图像堆栈计算得出的荧光团丰度图上,EGFP被强烈的绿色单体荧光掩盖,无法检测到EGFP。因此,当从用明亮且发射光谱宽泛的染料(如AO)共标记的弱荧光EGFP标记细胞器的图像中获取定量共定位信息时,需要格外谨慎。我们最终引入FM4 - 64/EGFP双色成像作为一种方法,用于对一群不同的具有融合能力的星形胶质细胞分泌囊泡进行成像。

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