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Multifocal plane microscopy for the study of cellular dynamics in three dimensions.

机译:多焦点平面显微镜用于研究三维细胞动力学。

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摘要

Fluorescence microscopy is an invaluable tool to investigate cellular trafficking pathways in live cells. For example, Total Internal Reflection Fluorescence (TIRF) microscopy has enabled high sensitivity visualization of trafficking events on the plasma membrane of a cell. Similarly, epifluorescence microscopy is a widely used imaging technique to study cellular dynamics inside a cell. However, tracking of cellular components that move in three dimensions, i.e. between different focal planes, is problematic. To enable tracking in three dimensions, typically multiple focal planes of a sample are sequentially imaged by changing the objective focus using a focusing device. However, the speed of image acquisition is limited with such focusing devices. Additionally, only one focal plane can be visualized at a given time. Therefore, important events that take place outside this focal plane can be missed. To facilitate the simultaneous visualization of multiple focal planes of a sample, multifocal plane microscopy has been developed during this research project. This has been achieved by a modification of the emission light path of a conventional microscope and by utilizing a multi-camera image acquisition format. A design of the excitation light path of a fluorescence microscope that allows for simultaneous TIRF and epifluorescence illumination is also presented in this thesis. This excitation scheme together with multifocal plane microscopy enables the simultaneous visualization of the events on the plasma membrane and inside a cell. To demonstrate the capabilities of this new imaging modality, a study has been conducted at the cellular level to understand the mechanism of antibody trafficking in three dimensions, specifically of immunoglobulin G as mediated by the neonatal Fc receptor, FcRn. This study has provided insight into the intracellular trafficking events on the recycling pathway preceding exocytosis of FcRn. Software tools were also developed for automated image acquisition and image processing. Developed using the object-oriented design philosophy, the image acquisition software package provides a flexible environment to integrate hardware components. The software tools for image processing utilize image pointers to organize and process the multifocal plane microscopy data.
机译:荧光显微镜是研究活细胞中细胞运输途径的宝贵工具。例如,全内反射荧光(TIRF)显微镜可以对细胞质膜上的运输事件进行高灵敏度可视化。同样,落射荧光显微镜是一种广泛使用的成像技术,用于研究细胞内部的细胞动力学。然而,跟踪在三个维度上(即,在不同焦平面之间)移动的细胞成分是有问题的。为了能够在三个维度上进行跟踪,通常使用聚焦装置通过改变物镜焦点来顺序成像样品的多个聚焦平面。但是,这种聚焦装置限制了图像获取的速度。另外,在给定时间只能看到一个焦平面。因此,可以错过在此焦平面外发生的重要事件。为便于同时显示样品的多个焦平面,在此研究项目期间已开发了多焦平面显微镜。这是通过修改常规显微镜的发射光路并利用多摄像机图像采集格式来实现的。本文还提出了允许同时进行TIRF和落射荧光照明的荧光显微镜激发光路的设计。这种激发方案与多焦平面显微镜一起可以同时观察质膜和细胞内部的事件。为了证明这种新的成像方式的功能,已在细胞水平上进行了一项研究,以了解抗体运输的三个方面的机制,特别是由新生儿Fc受体FcRn介导的免疫球蛋白G的运输。该研究提供了对FcRn胞吐作用之前再循环途径上的细胞内运输事件的见解。还开发了用于自动图像采集和图像处理的软件工具。使用面向对象的设计理念开发的图像采集软件包提供了灵活的环境来集成硬件组件。用于图像处理的软件工具利用图像指针来组织和处理多焦平面显微镜数据。

著录项

  • 作者

    Prabhat, Prashant.;

  • 作者单位

    The University of Texas at Dallas.;

  • 授予单位 The University of Texas at Dallas.;
  • 学科 Biology Cell.Engineering Electronics and Electrical.Engineering Biomedical.
  • 学位 Ph.D.
  • 年度 2008
  • 页码 163 p.
  • 总页数 163
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 康复医学;
  • 关键词

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