首页> 外文期刊>Cytometry, Part A: the journal of the International Society for Analytical Cytology >Imaging fluorescence detected linear dichroism of plant cell walls in laser scanning confocal microscope
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Imaging fluorescence detected linear dichroism of plant cell walls in laser scanning confocal microscope

机译:激光扫描共聚焦显微镜成像荧光检测植物细胞壁的线性二向色性

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Anisotropy carries important information on the molecular organization of biological samples. Its determination requires a combination of microscopy and polarization spectroscopy tools. The authors constructed differential polarization (DP) attachments; to a laser scanning microscope in order to determine physical quantities related to the anisotropic distribution of molecules in microscopic samples; here the authors focus on fluorescence-detected linear dichroism (FDLD). By modulating the linear polarization of the laser beam between two orthogonally polarized states and by using a demodulation circuit, the authors determine the associated transmitted and fluorescence intensity-difference signals, which serve the basis for LD (linear dichroism) and FDLD, respectively. The authors demonstrate on sections of Convallaria majalis root tissue stained with Acridin Orange that while (nonconfocal) LD images remain smeared and weak, FDLD images recorded in confocal mode reveal strong anisotropy of the cell wall. FDLD imaging is suitable for mapping the anisotropic distribution of transition dipoles in 3 dimensions. A mathematical model is proposed to account for the fiber-laminate ultrastructure of the cell wall and for the intercalation of the dye molecules in complex, highly anisotropic architecture.
机译:各向异性携带着有关生物样品分子结构的重要信息。其测定需要结合使用显微镜和偏振光谱学工具。作者构建了差分极化(DP)附件。为了确定与微观样品中分子的各向异性分布有关的物理量,使用激光扫描显微镜;在这里,作者专注于荧光检测线性二向色性(FDLD)。通过在两个正交偏振态之间调制激光束的线性偏振,并使用解调电路,作者确定了相关的透射和荧光强度差信号,它们分别用作LD(线性二向色性)和FDLD的基础。这组作者在用Acridin Orange染色的铃兰根部组织切片上证实,(非共聚焦的)LD图像仍然被涂片且微弱,以共聚焦模式记录的FDLD图像显示出细胞壁的强各向异性。 FDLD成像适合于绘制3维三维跃迁偶极子的各向异性分布。提出了一个数学模型来解释细胞壁的纤维层压超微结构以及复杂,高度各向异性的结构中染料分子的嵌入。

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