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Technique development in super-resolution fluorescence microscopy.

机译:超分辨率荧光显微镜技术的发展。

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摘要

I present three projects all of which involve innovations in fluorescence microscopy. First I present a microscopy method whereby the angular dependence of a fluorophore's emission pattern near a bare glass surface or metal-coated surface that supports surface plasmon resonance is measured. This technique involves altering the microscope optics to directly record (on a CCD camera) the intensity pattern at the objective's back focal plane. This intensity pattern directly maps the angular emission pattern of fluorescence. The experimental emission profile on both glass and aluminum-coated surfaces is anisotropic with a peak at either the critical angle or both the critical angle and the surface plasmon angle. The observed profiles on both glass and aluminum-coated surfaces are anisotropic and agree well with computer calculations.; Second I present a new fluorescence resonance energy transfer (FRET) method based on polarization that determines FRET using data from a single camera exposure, offering better time resolution of dynamic associations. Polarized FRET uses a simultaneous combination of excitation wavelengths from two orthogonally polarized sources, along with an emission channel tri-image splitter outfitted with appropriate polarizers, to concurrently excite and collect fluorescence from free donors, free acceptors, and FRET pairs. The pixel-by-pixel concentrations of all molecules can then be determined. Here I present the theory of polarized FRET and examine its feasibility through both theoretical investigation and experimental confirmation on mixtures of fluorescent proteins expressed in living cells.; Third, I present a method for directly measuring the depth and purity of the evanescent field used for fluorophore excitation in total internal reflection fluorescence (TIRF) microscopy. This technique involves microscopic observation of low refractive index, fluorescently labeled, spherical beads in an index-matched solution. With both the 1.45 NA and 1.65 NA objectives on the Olympus microscope the profile of the evanescent field fits well to a double exponential with 90% of the field represented by an exponential with a decay rate close to that expected for a pure evanescent field and 10% of the field represented by an exponential with a much longer decay constant attributed to scattering.
机译:我介绍了三个项目,所有这些项目都涉及荧光显微镜的创新。首先,我介绍了一种显微镜方法,该方法可以测量在支持表面等离子体共振的裸露玻璃表面或金属涂层表面附近的荧光团发射图的角度依赖性。该技术涉及更改显微镜光学器件,以直接记录(在CCD摄像机上)物镜后焦平面处的强度模式。该强度图案直接映射荧光的角发射图案。在玻璃和铝涂层表面上的实验发射曲线都是各向异性的,在临界角或在临界角和表面等离激元角上都有一个峰值。在玻璃和铝涂层表面上观察到的轮廓是各向异性的,并且与计算机计算非常吻合。其次,我提出了一种新的基于极化的荧光共振能量转移(FRET)方法,该方法使用一次摄影机曝光的数据确定FRET,从而提供更好的动态关联时间分辨率。偏振FRET使用来自两个正交偏振源的激发波长以及配备有适当偏振器的发射通道三像分光器的同时组合,来同时激发和收集来自自由供体,自由受体和FRET对的荧光。然后可以确定所有分子的逐像素浓度。在这里,我介绍了极化FRET的理论,并通过理论研究和对活细胞中表达的荧光蛋白混合物的实验验证,检验了其可行性。第三,我提出了一种在全内反射荧光(TIRF)显微镜中直接测量用于荧光团激发的van逝场的深度和纯度的方法。该技术涉及在折射率匹配溶液中显微镜观察低折射率,荧光标记的球形珠。在Olympus显微镜上使用1.45 NA和1.65 NA物镜时,field逝场的轮廓非常适合双指数,其中90%的场由指数表示,其衰减率接近于纯e逝场和10的衰减率。以指数表示的场的百分比,该指数具有更长的归因于散射的衰减常数。

著录项

  • 作者

    Mattheyses, Alexa Lynn.;

  • 作者单位

    University of Michigan.;

  • 授予单位 University of Michigan.;
  • 学科 Biophysics General.
  • 学位 Ph.D.
  • 年度 2005
  • 页码 102 p.
  • 总页数 102
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物物理学;
  • 关键词

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