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通过双标记光开关荧光蛋白的高对比度荧光偏振显微镜。

High contrast fluorescence polarization microscopy through double tagged photoswitchable fluorescent proteins.

作者信息

Münker Lukas J, Hohgardt Manuel, Albrecht Andreas, Pfennig Dominik, Tegtmeier Jan S, Holz Andreas, Zagrebelsky Marta, Korte Martin, Walla Peter J

机构信息

Technical University of Braunschweig, Braunschweig, Germany.

Helmholtz Centre for Infection Research, Braunschweig, Germany.

出版信息

Npj Imaging. 2025 Jul 2;3(1):31. doi: 10.1038/s44303-025-00094-y.

Abstract

We demonstrate that rigid anchoring of fluorescent proteins through double tagging (FPs) in living cells can significantly enhance the contrast in fluorescence polarization microscopy (FPM) by locking the transition dipole moment orientations to the sample's structures. We applied double tagging of reversibly photoswitchable FPs (dt-rsFPs) to membranes and present a novel camera frame-separated switching pulse scheme that allows effective narrowing of the angle range of excited dt-FP also in living cells (frame-separated excitation polarization angle narrowing, FrExPAN). The principle of rigid anchoring allows specific selection of signals from different structural cell parts with slightly different orientations and is broadly applicable. FrExPAN imaging with dt-rsFPs double-tagged to membranes of living HeLa cells and living hippocampal neurons is demonstrated. We discuss potential implications for orientational contrast imaging as well as super-resolution by polarization demodulation (SPoD) methods.

摘要

我们证明,通过在活细胞中对荧光蛋白进行双标记(FPs)来实现刚性锚定,可通过将跃迁偶极矩方向锁定到样品结构上,显著增强荧光偏振显微镜(FPM)中的对比度。我们将可逆光开关荧光蛋白的双标记(dt-rsFPs)应用于细胞膜,并提出了一种新颖的相机帧分离切换脉冲方案,该方案也能在活细胞中有效缩小激发dt-FP的角度范围(帧分离激发偏振角变窄,FrExPAN)。刚性锚定原理允许从方向略有不同的不同细胞结构部分中特异性选择信号,并且具有广泛的适用性。本文展示了用dt-rsFPs双标记活HeLa细胞和活海马神经元细胞膜的FrExPAN成像。我们讨论了其对取向对比度成像以及通过偏振解调(SPoD)方法实现超分辨率的潜在意义。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/81e2/12222721/290965fbea54/44303_2025_94_Fig1_HTML.jpg

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