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Confocal and two-photon microscopy: Image enhancement.

机译:共聚焦和双光子显微镜:图像增强。

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摘要

Confocal and two-photon microcopy have become essential tools in biological research and today many investigations are not possible without their help. The valuable advantage that these two techniques offer is the ability of optical sectioning. Optical sectioning makes it possible to obtain 3D visualization of the structures, and hence, valuable information of the structural relationships, the geometrical, and the morphological aspects of the specimen.;This thesis presents an investigation and study of image enhancement. The goal of this thesis was approached in two different directions. Initially, we investigated the sources of the imperfections. We propose methods to eliminate or minimize aberrations introduced during the image acquisition by optimizing the acquisition conditions. The impact on the resolution as a result of using a coverslip the thickness of which is mismatched with the one that the objective lens is designed for was shown and a novel technique was introduced in order to define the proper value on the correction collar of the lens. The amount of spherical aberration with regard to the numerical aperture of the objective lens was investigated and it was shown that, based on the purpose of our imaging tasks, different numerical apertures must be used. The deformed beam cross section of the single-photon excitation source was corrected and the enhancement of the resolution and image quality was shown. Furthermore, the dependency of the scattered light on the excitation wavelength was shown empirically.;In the second part, we continued the study of the image enhancement process by de-convolution techniques. Although deconvolution algorithms are used widely to improve the quality of the images, how well a deconvolution algorithm responds highly depends on the point spread function (PSF) of the imaging system applied to the algorithm and the level of its accuracy. We investigated approaches that can be done in order to obtain more precise PSF. Novel methods to improve the pattern of the PSF and reduce the noise are proposed. Furthermore, multiple sources to extract the PSFs of the imaging system are introduced and the empirical deconvolution results by using each of these PSFs are compared together. The results confirm that a greater improvement attained by applying the in situ PSF during the deconvolution process.;The achievable lateral and axial resolutions by confocal and two-photon microscopy, similar to other optical imaging systems, are both defined by the diffraction theorem. Any aberration and imperfection present during the imaging results in broadening of the calculated theoretical resolution, blurring, geometrical distortions in the acquired images that interfere with the analysis of the structures, and lower the collected fluorescence from the specimen. The aberrations may have different causes and they can be classified by their sources such as specimen-induced aberrations, optics-induced aberrations, illumination aberrations, and misalignment aberrations.
机译:共聚焦和双光子显微镜已成为生物学研究中必不可少的工具,如今,没有它们的帮助,许多研究是不可能的。这两种技术提供的宝贵优势是光学切片的能力。光学切片使获得3D可视化的结构成为可能,因此,可以获得标本的结构关系,几何和形态方面的有价值的信息。;本文对图像增强进行了研究和研究。本文的目的是从两个不同的方向来实现的。最初,我们调查了缺陷的来源。我们提出了通过优化采集条件来消除或最小化在图像采集过程中引入的像差的方法。显示了使用盖玻片厚度与物镜设计不匹配的盖玻片对分辨率的影响,并介绍了一种新技术以在镜片的校正环上定义合适的值。研究了关于物镜数值孔径的球差量,结果表明,基于我们成像任务的目的,必须使用不同的数值孔径。校正了单光子激发源的变形光束横截面,并显示了分辨率和图像质量的提高。此外,还通过经验证明了散射光对激发波长的依赖性。第二部分,我们继续通过反卷积技术研究图像增强过程。尽管反卷积算法被广泛用于提高图像质量,但是反卷积算法的响应良好程度取决于应用于该算法的成像系统的点扩展函数(PSF)及其准确性。我们研究了可以获取更精确的PSF的方法。提出了改善PSF模式并降低噪声的新方法。此外,介绍了提取成像系统PSF的多种来源,并将使用这些PSF中的每一个的经验去卷积结果进行了比较。结果证实,通过在反卷积过程中应用原位PSF可获得更大的改进。共聚焦和双光子显微镜可实现的横向和轴向分辨率,与其他光学成像系统类似,均由衍射定理定义。成像期间出现的任何像差和瑕疵都会导致计算出的理论分辨率变宽,所采集图像中的模糊,几何畸变,从而干扰结构分析,并降低从样品中收集的荧光。像差可能具有不同的原因,并且可以按其来源对它们进行分类,例如样品引起的像差,光学引起的像差,照明像差和未对准像差。

著录项

  • 作者

    Kefayati, Sarah.;

  • 作者单位

    Brock University (Canada).;

  • 授予单位 Brock University (Canada).;
  • 学科 Physics Optics.
  • 学位 M.Sc.
  • 年度 2008
  • 页码 85 p.
  • 总页数 85
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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