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生物组织中内源性结构蛋白的三维高分辨率二次谐波生成成像

Three-dimensional high-resolution second-harmonic generation imaging of endogenous structural proteins in biological tissues.

作者信息

Campagnola Paul J, Millard Andrew C, Terasaki Mark, Hoppe Pamela E, Malone Christian J, Mohler William A

机构信息

Department of Physiology, University of Connecticut Health Center, Farmington, Connecticut 06030, USA.

出版信息

Biophys J. 2002 Jan;82(1 Pt 1):493-508. doi: 10.1016/S0006-3495(02)75414-3.

Abstract

We find that several key endogenous protein structures give rise to intense second-harmonic generation (SHG)-nonabsorptive frequency doubling of an excitation laser line. Second-harmonic imaging microscopy (SHIM) on a laser-scanning system proves, therefore, to be a powerful and unique tool for high-resolution, high-contrast, three-dimensional studies of live cell and tissue architecture. Unlike fluorescence, SHG suffers no inherent photobleaching or toxicity and does not require exogenous labels. Unlike polarization microscopy, SHIM provides intrinsic confocality and deep sectioning in complex tissues. In this study, we demonstrate the clarity of SHIM optical sectioning within unfixed, unstained thick specimens. SHIM and two-photon excited fluorescence (TPEF) were combined in a dual-mode nonlinear microscopy to elucidate the molecular sources of SHG in live cells and tissues. SHG arose not only from coiled-coil complexes within connective tissues and muscle thick filaments, but also from microtubule arrays within interphase and mitotic cells. Both polarization dependence and a local symmetry cancellation effect of SHG allowed the signal from species generating the second harmonic to be decoded, by ratiometric correlation with TPEF, to yield information on local structure below optical resolution. The physical origin of SHG within these tissues is addressed and is attributed to the laser interaction with dipolar protein structures that is enhanced by the intrinsic chirality of the protein helices.

摘要

我们发现,几种关键的内源性蛋白质结构会产生强烈的二次谐波产生(SHG)——激发激光线的非吸收性倍频。因此,激光扫描系统上的二次谐波成像显微镜(SHIM)被证明是用于活细胞和组织结构的高分辨率、高对比度三维研究的强大且独特的工具。与荧光不同,SHG不存在固有的光漂白或毒性,也不需要外源性标记。与偏振显微镜不同,SHIM在复杂组织中提供内在的共焦性和深度切片。在本研究中,我们展示了SHIM在未固定、未染色的厚标本中的光学切片清晰度。SHIM和双光子激发荧光(TPEF)在双模式非线性显微镜中相结合,以阐明活细胞和组织中SHG的分子来源。SHG不仅来自结缔组织和肌肉粗肌丝中的卷曲螺旋复合物,还来自间期和有丝分裂细胞中的微管阵列。SHG的偏振依赖性和局部对称性抵消效应都使得通过与TPEF的比率相关性对产生二次谐波的物质的信号进行解码,从而获得低于光学分辨率的局部结构信息。本文探讨了这些组织中SHG的物理起源,并将其归因于激光与偶极蛋白质结构的相互作用,这种相互作用因蛋白质螺旋的固有手性而增强。

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