生成适合核蛋白超分辨率成像的α gfp纳米体

N. Bachmann
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引用次数: 0

摘要

单分子定位显微镜(SMLM)技术的出现使得细胞成像的分辨率远远超过衍射障碍成为可能。然而,通常用一抗标记感兴趣蛋白(PoI),并用携带荧光团的二抗标记这一蛋白的方法,会导致PoI信号的显著位移。本文描述了α gfp纳米体的生成和应用,该纳米体通过其缩小的尺寸和直接荧光团标记,导致信号和PoI的共定位更高,并符合核蛋白的dSTORM成像。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Generation of αGFP-nanobodies suitable for super-resolution imaging of nuclear proteins
The emergence of single molecule localization microscopy (SMLM) techniques made the imaging of cells at resolutions far beyond the diffraction barrier possible. However, the usual approach of tagging a protein of interest (PoI) with a primary antibody, and tagging this one with a fluorophore-carrying secondary antibody, introduces a significant displacement of the signal from the PoI. Here, the generation and application of an αGFP-nanobody is described which, through its reduced size and direct fluorophore labeling, leads to a much higher co-localization of signal and PoI and qualifies for dSTORM imaging of nuclear proteins.
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